ABSTRACT
BACKGROUND: Target enrichment is a critical component of targeted deep next-generation sequencing for the cost-effective and sensitive detection of mutations, which is predominantly performed by either hybrid selection or PCR. Despite the advantages of efficient enrichment, PCR-based methods preclude the identification of PCR duplicates and their subsequent removal. Recently, this limitation was overcome by assigning a unique molecular identifier(UMI) to each template molecule. Currently, several commercial library construction kits based on PCR enrichment are available for UMIs, but there have been no systematic studies to compare their performances. In this study, we evaluated and compared the performances of five commercial library kits from four vendors: the Archer® Reveal ctDNA™ 28 Kit, NEBNext Direct® Cancer HotSpot Panel, Nugen Ovation® Custom Target Enrichment System, Qiagen Human Comprehensive Cancer Panel(HCCP), and Qiagen Human Actionable Solid Tumor Panel(HASTP). RESULTS: We evaluated and compared the performances of the five kits using 50 ng of genomic DNA for the library construction in terms of the library complexity, coverage uniformity, and errors in the UMIs. While the duplicate rates for all kits were dramatically decreased by identifying unique molecules with UMIs, the Qiagen HASTP achieved the highest library complexity based on the depth of unique coverage indicating superb library construction efficiency. Regarding the coverage uniformity, the kits from Nugen and NEB performed the best followed by the kits from Qiagen. We also analyzed the UMIs, including errors, which allowed us to adjust the depth of unique coverage and the length required for sufficient complexity. Based on these comparisons, we selected the Qiagen HASTP for further performance evaluations. The targeted deep sequencing method based on PCR target enrichment combined with UMI tagging sensitively detected mutations present at a frequency as low as 1% using 6.25 ng of human genomic DNA as the starting material. CONCLUSION: This study is the first systematic evaluation of commercial library construction kits for PCR-based targeted deep sequencing utilizing UMIs. Because the kits displayed significant variability in different quality metrics, our study offers a practical guideline for researchers to choose appropriate options for PCR-based targeted sequencing and useful benchmark data for evaluating new kits.
Subject(s)
Biomarkers/analysis , DNA/analysis , Gene Library , High-Throughput Nucleotide Sequencing/methods , Polymerase Chain Reaction/methods , Reagent Kits, Diagnostic/standards , DNA/isolation & purification , High-Throughput Nucleotide Sequencing/standards , Humans , Polymerase Chain Reaction/standardsABSTRACT
Galactinol synthase (GS, EC 2.4.1.123) catalyzes the transfer of a galactosyl residue from UDP-galactose to myo-inositol to synthesize galactinol, a precursor for raffinose family oligosaccharides (RFO) biosynthesis. Screening, a cDNA library constructed with RNA isolated from developing lentil seeds, with partial GS genes resulted in identification of cDNA clones for two isoforms of GS, LcGolS1 (1336 bp, ORF-1002 bp, 334 amino acids) and LcGolS2 (1324bp, ORF-975bp, 325 amino acids) with predicted molecular weights of 38.7 kDa and 37.6 kDa, respectively. During lentil seed development, LcGolS1 transcripts showed higher accumulation during 26-32 days after flowering (DAF) corresponding to seed desiccation, while LcGolS2 showed maximum accumulation at 24 DAF, prior to increase in LcGolS1 transcripts. GS enzyme activity was maximum at 26 and 28 DAF and corresponded to galactinol accumulation, which also increased rapidly at 22 DAF with maximum accumulation at 26 DAF. Substrates for GS activity, myo-inositol and glucose/galactose were present in high concentrations during early stages of seed development but gradually decreased from 20 DAF to 32 DAF when galactinol concentration increased coinciding with increased GS enzyme activity.
Subject(s)
Galactosyltransferases/metabolism , Lens Plant/enzymology , Plant Proteins/metabolism , Seeds/enzymology , Seeds/growth & development , Cloning, Molecular , DNA, Complementary , Disaccharides/metabolism , Galactosyltransferases/chemistry , Galactosyltransferases/genetics , Gene Expression Regulation, Plant , Gene Library , Isoenzymes/genetics , Isoenzymes/metabolism , Lens Plant/genetics , Lens Plant/growth & development , Phylogeny , Plant Proteins/genetics , Polymerase Chain Reaction/methods , Polymerase Chain Reaction/standards , Protein Conformation , Reference Standards , Reproducibility of Results , Seeds/geneticsABSTRACT
Timely diagnosis of the nematode Angiostrongylus vasorum in dogs is important in view of severe and permanent lung and cardiovascular lesions that may occur. The performance of the classical Baermann coprological method was compared with ELISAs for the serological detection of circulating antigen and specific antibodies and with Polymerase chain reaction (PCR) performed on EDTA blood, feces and tracheal swabs of serial samples from experimentally inoculated dogs over 13 weeks post inoculation (wpi) (n = 16) and following anthelmintic treatment (n = 6). Patency was observed from 6.7 to 7.6 wpi in all dogs, Baermann results were then mostly positive (116/119, 97%) during the patent period, with wide variations in the numbers of first stage larvae numbers. Blood PCR was tested positive on 1-2 occasions in 11/16 dogs in the pre-patent period, while all tested positive by antibody-detection ELISA by 6 wpi. The proportion of dogs testing positive by fecal PCR and antigen-detection ELISA rose early in the patent period. Tracheal swabs were occasionally DNA-positive in 3/16 dogs starting from 10 wpi. Following treatment, larval excretion stopped within 3 weeks and blood PCR results became negative within 1 week (5/6 dogs), while 4/6 dogs were positive for parasite DNA in tracheal swabs. Parasite antigen and specific antibodies both persisted in the blood for 3-9 weeks after treatment, with average optical densities and the proportion of positive dogs falling gradually, while results using other tests were much more variable. Results indicate that the earliest and most consistent results are obtained by the ELISAs, which can also be used for monitoring dogs after anthelmintic treatment.
Subject(s)
Anthelmintics/therapeutic use , Dog Diseases/diagnosis , Dog Diseases/drug therapy , Feces/parasitology , Strongylida Infections/drug therapy , Strongylida Infections/veterinary , Angiostrongylus/immunology , Angiostrongylus/physiology , Animals , Antibodies, Helminth/blood , Dogs , Enzyme-Linked Immunosorbent Assay/standards , Enzyme-Linked Immunosorbent Assay/veterinary , Polymerase Chain Reaction/standards , Polymerase Chain Reaction/veterinary , Sensitivity and Specificity , Strongylida Infections/diagnosisABSTRACT
A novel immobilization approach involving binding of preformed streptavidin/biotinylated oligonucleotide conjugates onto surfaces coated with biotinylated bovine serum albumin is presented. Microarrays prepared according to the proposed method were compared, in terms of detection sensitivity and specificity, with other immobilization schemes employing coupling of biotinylated oligonucleotides onto directly adsorbed surface streptavidin, or sequential coupling of streptavidin and biotinylated oligonucleotides onto a layer of adsorbed biotinylated bovine serum albumin. A comparison was performed employing biotinylated oligonucleotides corresponding to wild- and mutant-type sequences of seven single point mutations of the BRCA1 gene. With respect to the other immobilization protocols, the proposed oligonucleotide immobilization approach offered the highest hybridization signals (at least 5 times higher) and permitted more elaborative washings, thus providing considerably higher discrimination between complimentary and non-complementary DNA sequences for all mutations tested. In addition, the hybridization kinetics were significantly enhanced compared to two other immobilization protocols, permitting PCR sample analysis in less than 40 min. Thus, the proposed oligonucleotide immobilization approach offered improved detection sensitivity and discrimination ability along with considerably reduced analysis time, and it is expected to find wide application in DNA mutation detection.
Subject(s)
Biotin/chemistry , DNA Mutational Analysis/standards , Mutation , Oligonucleotide Array Sequence Analysis/standards , Oligonucleotides/chemistry , Streptavidin/chemistry , Animals , BRCA1 Protein/chemistry , BRCA1 Protein/genetics , Base Pairing , Biotinylation , Cattle , DNA Mutational Analysis/economics , Humans , Oligonucleotide Array Sequence Analysis/economics , Oligonucleotide Array Sequence Analysis/instrumentation , Polymerase Chain Reaction/standards , Protein Binding , Sensitivity and Specificity , Serum Albumin, Bovine/chemistry , Time FactorsABSTRACT
Las metalo-βeta-lactamasas (MBL) que producen las bacterias gram-negativas son un creciente problema de salud pública en todo el mundo. Las pruebas de detección para la identificación rápida y específica de estos patógenos son esenciales y deben ser incluídas entre los diagnósticos de rutina de los laboratorios. Este estudio tiene como objetivo determinar la frecuencia de MBL en aislamientos de Pseudomona aeruginosa resistentes a carbapenem y evaluar la precisión de diferentes pruebas en la detección de la producción de MBL. Entre enero de 2001 y diciembre de 2008 un total de 142 cepas de P. aeruginosa no susceptibles a imipenem fueron aisladas de muestras clínicas provenientes de pacientes hospitalizados. Estas cepas fueron examinadas por PCR, prueba de MBL-E, prueba de sinergia de doble disco (DDS), y prueba de disco combinado (DC). La concentración inhibitoria mínima (CIM; g/ml) se determinó mediante dilución en agar. Se realizó electroforesis en gel de campo pulsado (PFGE) a todas las muestras. La secuenciación se realizó para confirmar y definir la variante de MBL y subtipo. Por PCR y análisis de secuencia de ADN, 93 cepas fueron confirmadas como positivas para MBL. A su vez, 91 cepas fueron confirmadas para el gen blaSPM-1, 1 cepa para el gen bla IMP-1, y 1 cepa para el gen bla IMP-16. La prueba de PFGE muestra un patrón clonal. Se evaluó la sensibilidad, especificidad, valores predictivos positivos y negativos para todas las pruebas. El ensayo DDS (CAZ-MPA) fue el método óptimo para la detección de la producción de MBL en las cepas de P. aeruginosa. Sin embargo, los resultados del ensayo de DC (IMP/EDTA) mostraron una estrecha concordancia con los de la DDS. Adicionalmente, el ensayo de DC permitió una interpretación más objetiva de los resultados, no requiriendo el uso de una sustancia tóxica
Metallo-βeta-lactamase (MBL)-producing gram-negative bacteria are an increasing public health concern worldwide. Screening tests for the rapid and specific identification of these pathogens are essential, and should be included among routine diagnostics in laboratories. This study aimed to determine the MBL frequency among carbapenem-resistant Pseudomonas aeruginosa isolates, and to evaluate the accuracy of different tests in screening for MBL production. From January 2001 to December 2008, a total of 142 imipenem-non-susceptible P. aeruginosa strains were isolated from distinct clinical samples from hospitalized patients. These isolates were examined by PCR, MBL E-test, double-disk synergy test (DDST), and combined disk (CD) test. The minimal inhibitory concentration (MIC; μg/mL) was determined by agar dilution, and pulsed field gel electrophoresis (PFGE) was performed on all samples. Sequencing was performed to confirm and define the MBL variant and subtype. Using PCR and DNA sequence analysis, 93 strains were confirmed positive for MBLs, 91 strains for the blaSPM-1 gene, 1 strain for the blaIMP-1 gene, and 1 strain for the blaIMP-16 gene. PFGE displayed a clonal pattern. The sensitivities, specificities, positive and negative predictive values were evaluated for all tests. The DDST assay (CAZ-MPA) was the optimal method for screening MBL production in P. aeruginosa strains. However, the results of the CD assay (IMP/EDTA) showed close agreement with those of the DDST. In addition, the CD assay allowed a more objective interpretation and did not require the use of a toxic substance
Subject(s)
Humans , Male , Female , Pseudomonas aeruginosa , Pseudomonas aeruginosa/isolation & purification , Carbapenems/metabolism , Carbapenems/therapeutic use , Bacteria/isolation & purification , Public Health/methods , Polymerase Chain Reaction/methods , Polymerase Chain Reaction/standards , Polymerase Chain Reaction , Drug Synergism , ROC CurveABSTRACT
Apical leaf curl disease has emerged as a new disease in potato during the last decade in India due to a change in planting date and an increased whitefly population. Its incidence is on the rise threatening the cultivation of potato across the country. Hence, a PCR assay was developed for the detection of Tomato leaf curl New Delhi virus-potato (ToLCNDV-Potato) which is the causal agent of apical leaf curl disease in potato. Primers specific to the coat protein (AV1) and replicase (AC1) gene regions were designed and used for standardization of the PCR. Some of the primers (LCVCPF1/LCVCPR1, LCVREPF2/LCVREPR2, LCrep1F/LCrep2R) could detect the virus in 2.4-0.24pg of total DNA of infected plant. A duplex PCR assay was optimized with the selected coat protein gene specific primers and primers specific to potato urease gene, a housekeeping gene served as an internal check. The suitability of these primers was examined for detection of the virus in 80 potato apical leaf curl disease samples from 11 different potato growing states of India and also from micro-plants grown in tissue culture. The selected coat protein primer pair (LCVCPF1/LCVCPR1) was found to be conserved in all 80 isolates except for a few isolates, which had a single nucleotide substitution in the forward primer sequence. These substitutions did not interfere with amplification of the coat protein gene. The primers could detect the virus using a print-capture PCR assay both in the presence and absence of an internal control. These results indicate the robustness of the PCR assay for virus indexing of mother stocks in the seed production system.
Subject(s)
Begomovirus/isolation & purification , Plant Diseases/virology , Polymerase Chain Reaction/methods , Solanum tuberosum/virology , Virology/methods , Capsid Proteins/genetics , DNA Primers/genetics , India , Plant Proteins/genetics , Polymerase Chain Reaction/standards , Reference Standards , Sensitivity and Specificity , Urease/genetics , Virology/standardsABSTRACT
BACKGROUND: Conventional methods for detecting fungi in nail specimens are either nonspecific (microscopy) or insensitive (culture). Recently, PCR has been used to improve sensitivity in detecting the causative fungi in nail specimens from patients with suspected onychomycosis. AIM: To compare the detection rates of PCR with those of microscopy (with potassium hydroxide; KOH) and culture for dermatophytes in nail specimens from patients with suspected onychomycosis. METHODS: In total, 120 patients with clinically suspected onychomycosis were recruited, and using a topoisomerase II-based PCR, we compared the detection rate of dermatophytes for the three methods. RESULTS: KOH microscopy, culture and PCR respectively yielded positive rates of 35 (29.2%), 12 (10%) and 48 (40%), and negative rates of 85 (70.8%), 108 (90%) and 72 (60%). Two culture-positive specimens were not detected by PCR, but PCR picked up 38 specimens missed by culture. Of the 35 specimens that were microscopy-positive, 12 grew dermatophytes and 23 nondermatophytes. CONCLUSIONS: This study demonstrates that PCR has a higher positive and lower negative rate for detection of dermatophytes compared with KOH microscopy or culture. We suggest that PCR should be used as a complementary method for confirmation of clinically suspected dermatophytic onychomycosis.
Subject(s)
Arthrodermataceae/isolation & purification , Onychomycosis/diagnosis , Polymerase Chain Reaction/standards , Adolescent , Adult , Aged , Aged, 80 and over , Child , Female , Humans , Male , Microscopy , Middle Aged , Onychomycosis/microbiology , Polymerase Chain Reaction/methods , Prospective Studies , Sensitivity and Specificity , Young AdultABSTRACT
BACKGROUND: Gastrointestinal stromal tumors (GIST) represent the most common mesenchymal tumors of the gastrointestinal tract. About 85% carry an activating mutation in the KIT or PDGFRA gene. Approximately 10% of GIST are so-called wild type GIST (wt-GIST) without mutations in the hot spots. In the present study we evaluated appropriate reference genes for the expression analysis of formalin-fixed, paraffin-embedded and fresh frozen samples from gastrointestinal stromal tumors. We evaluated the gene expression of KIT as well as of the alternative receptor tyrosine kinase genes FLT3, CSF1-R, PDGFRB, AXL and MET by qPCR. wt-GIST were compared to samples with mutations in KIT exon 9 and 11 and PDGFRA exon 18 in order to evaluate whether overexpression of these alternative RTK might contribute to the pathogenesis of wt-GIST. RESULTS: Gene expression variability of the pooled cDNA samples is much lower than the single reverse transcription cDNA synthesis. By combining the lowest variability values of fixed and fresh tissue, the genes POLR2A, PPIA, RPLPO and TFRC were chosen for further analysis of the GIST samples. Overexpression of KIT compared to the corresponding normal tissue was detected in each GIST subgroup except in GIST with PDGFRA exon 18 mutation. Comparing our sample groups, no significant differences in the gene expression levels of FLT3, CSF1R and AXL were determined. An exception was the sample group with KIT exon 9 mutation. A significantly reduced expression of CSF1R, FLT3 and PDGFRB compared to the normal tissue was detected. GIST with mutations in KIT exon 9 and 11 and in PDGFRA exon 18 showed a significant PDGFRB downregulation. CONCLUSIONS: As the variability of expression levels for the reference genes is very high comparing fresh frozen and formalin-fixed tissue there is a strong need for validation in each tissue type. None of the alternative receptor tyrosine kinases analyzed is associated with the pathogenesis of wild-type or mutated GIST. It remains to be clarified whether an autocrine or paracrine mechanism by overexpression of receptor tyrosine kinase ligands is responsible for the tumorigenesis of wt-GIST.
Subject(s)
Gastrointestinal Stromal Tumors/genetics , Gene Expression Profiling , Gene Expression Regulation, Neoplastic , Polymerase Chain Reaction , Proto-Oncogene Proteins c-kit/genetics , Receptor Protein-Tyrosine Kinases/genetics , DNA, Complementary/genetics , Gastrointestinal Stromal Tumors/pathology , Gene Expression Profiling/standards , Genes , Humans , Mutation , Polymerase Chain Reaction/standards , Proto-Oncogene Proteins/genetics , Proto-Oncogene Proteins c-met/genetics , RNA/isolation & purification , Receptor, Macrophage Colony-Stimulating Factor/genetics , Receptor, Platelet-Derived Growth Factor beta/genetics , Reference Standards , fms-Like Tyrosine Kinase 3/genetics , Axl Receptor Tyrosine KinaseABSTRACT
BACKGROUND: We have previously isolated a thermolabile nuclease specific for double-stranded DNA from industrial processing water of Northern shrimps (Pandalus borealis) and developed an application of the enzyme in removal of contaminating DNA in PCR-related technologies. METHODOLOGY/PRINCIPAL FINDINGS: A 43 kDa nuclease with a high specific activity of hydrolysing linear as well as circular forms of DNA was purified from hepatopancreas of Northern shrimp (Pandalus borealis). The enzyme displayed a substrate preference that was shifted from exclusively double-stranded DNA in the presence of magnesium to also encompass significant activity against single-stranded DNA when calcium was added. No activity against RNA was detected. Although originating from a cold-environment animal, the shrimp DNase has only minor low-temperature activity. Still, the enzyme was irreversibly inactivated by moderate heating with a half-life of 1 min at 65 degrees C. The purified protein was partly sequenced and derived oligonucleotides were used to prime amplification of the encoding cDNA. This cDNA sequence revealed an open reading frame encoding a 404 amino acid protein containing a signal peptide. By sequence similarity the enzyme is predicted to belong to a family of DNA/RNA non-specific nucleases even though this shrimp DNase lacks RNase activity and is highly double-strand specific in some respects. These features are in agreement with those previously established for endonucleases classified as similar to the Kamchatka crab duplex-specific nuclease (Par_DSN). Sequence comparisons and phylogenetic analyses confirmed that the Northern shrimp nuclease resembles the Par_DSN-like nucleases and displays a more distant relationship to the Serratia family of nucleases. CONCLUSIONS/SIGNIFICANCE: The shrimp nuclease contains enzyme activity that may be controlled by temperature or buffer compositions. The double-stranded DNA specificity, as well as the thermolabile feature, strengthens its potential for in vitro applications.
Subject(s)
Deoxyribonucleases/metabolism , Pandalidae/enzymology , Polymerase Chain Reaction/methods , Animals , Base Sequence , Calcium/pharmacology , DNA/metabolism , DNA, Complementary , DNA, Single-Stranded/metabolism , Magnesium/pharmacology , Pandalidae/genetics , Phylogeny , Polymerase Chain Reaction/standards , Substrate Specificity , TemperatureABSTRACT
Most nucleic acid-based technologies rely upon sequence recognition between an oligonucleotide and its nucleic acid target. With the aim of improving hybridization by decreasing electrostatic repulsions between the negatively charged strands, novel modified oligonucleotides named Zip nucleic acids (ZNAs) were recently developed. ZNAs are oligonucleotide-oligocation conjugates whose global charge is modulated by the number of cationic spermine moieties grafted on the oligonucleotide. It was demonstrated that the melting temperature of a hybridized ZNA is easily predictable and increases linearly with the length of the oligocation. Furthermore, ZNAs retain the ability to discriminate between a perfect match and a single base-pair-mismatched complementary sequence. Using quantitative PCR, we show here that ZNAs are specific and efficient primers displaying an outstanding affinity toward their genomic target. ZNAs are particularly efficient at low magnesium concentration, low primer concentrations and high annealing temperatures, allowing to improve the amplification in AT-rich sequences and potentially multiplex PCR applications. In reverse transcription experiments, ZNA gene-specific primers improve the yield of cDNA synthesis, thus increasing the accuracy of detection, especially for genes expressed at low levels. Our data suggest that ZNAs exhibit faster binding kinetics than standard and locked nucleic acid-containing primers, which could explain why their target recognition is better for rare targets.
Subject(s)
DNA Primers , Polymerase Chain Reaction , Reverse Transcription , AT Rich Sequence , Polymerase Chain Reaction/standardsABSTRACT
The aim of this study was to determine the prevalence and the transmission routes of Arcobacter spp. in sows and their offspring on a breeding farm. Twelve Arcobacter-positive sows and their litters were studied for this purpose. Analysis of rectal samples showed a high prevalence of Arcobacter spp. among the sows (approximately 42% of the sows carried one or more Arcobacter species). Intermittent excretion of one particular species and shifts in excretion from one species to another were observed in individual animals over time. The detection of Arcobacter spp. in amniotic fluid of the sows and in rectal samples from newborn piglets (ranging from 38.5-83.3% per litter), as well as the high similarity between PFGE profiles of Arcobacter isolates from sows and their respective newborns indicated the existence of an intra-uterine transmission route for Arcobacter spp. Specific antibodies against Arcobacter spp. were detected in colostrum by Western blot. At 2 weeks of age, only a few piglets were positive for Arcobacter. The reappearance of Arcobacter in these piglets at Week 3 and the shift in the Arcobacter species detected (from a prominent presence of A. cryaerophilus at birth to the presence of A. skirrowii and A. butzleri at 3 weeks after birth) showed that a post-natal infection route from their mothers, newcomers or the environment to the piglets existed. Thus, in this manuscript the transmission of Arcobacter spp. (both vertical and horizontal) from carrying sows to their offspring is demonstrated.
Subject(s)
Arcobacter , Disease Transmission, Infectious/veterinary , Gram-Negative Bacterial Infections/veterinary , Infectious Disease Transmission, Vertical/veterinary , Swine Diseases/microbiology , Swine Diseases/transmission , Amniotic Fluid/microbiology , Animals , Antibodies, Bacterial/analysis , Arcobacter/classification , Arcobacter/genetics , Arcobacter/isolation & purification , Blotting, Western/veterinary , Colostrum/immunology , DNA Primers/chemistry , DNA, Bacterial/chemistry , Electrophoresis, Gel, Pulsed-Field/methods , Electrophoresis, Gel, Pulsed-Field/veterinary , Female , Gram-Negative Bacterial Infections/epidemiology , Gram-Negative Bacterial Infections/microbiology , Gram-Negative Bacterial Infections/transmission , Polymerase Chain Reaction/methods , Polymerase Chain Reaction/standards , Polymerase Chain Reaction/veterinary , Rectum/microbiology , Sensitivity and Specificity , Swine Diseases/epidemiology , Time FactorsABSTRACT
In our laboratory, we have developed methods in real-time detection and quantitative-polymerase chain reaction (Q-PCR) to analyse the relative levels of gene expression in post mortem brain tissues. We have then applied this method to examine differences in gene activity between normal white matter (NWM) and plaque tissue from multiple sclerosis (MS) patients. Genes were selected based on their association with pathology and through identification by previously conducted global gene expression analysis. Plaque tissue was obtained from secondary progressive (SP) patients displaying chronic active, as well as acute pathologies; while NWM from the same location was obtained from age- and sex-matched controls (normal patients). In this study, we used both SYBR Green I supplementation and commercially available mixes to assess both comparative and absolute levels of gene activity. The results of both methods compared favourably for four of the five genes examined (P < 0.05, Pearsons), while differences in gene expression between chronic active and acute pathologies were also identified. For example, a >50-fold increase in osteopontin (Spp1) and inositol 1-4-5 phosphate 3 kinase B (Itpkb) levels in acute plaques contrasted with the 5-fold or less increase in chronic active plaques (P < 0.05, unpaired t test). By contrast, there was no significant difference in the levels of the MS marker and calcium-dependent protease (Calpain, Capns1) in MS plaque tissue. In summary, Q-PCR analysis using SYBR Green I has allowed us to economically obtain what may be clinically significant information from small amounts of the CNS, providing an opportunity for further clinical investigations.
Subject(s)
Gene Expression Profiling/methods , Multiple Sclerosis/genetics , Multiple Sclerosis/pathology , Polymerase Chain Reaction/methods , Female , Gene Dosage , Gene Expression Profiling/standards , Gene Expression Regulation , Genetic Markers , Humans , Male , Middle Aged , Polymerase Chain Reaction/standards , Postmortem Changes , Reproducibility of ResultsABSTRACT
We have developed a telomerase assay that can quickly and accurately rank the ability of molecules to inhibit telomerase activity. It is based on the method of Orlando and co-workers which utilizes PicoGreen to detect dsDNA formed during the polymerase chain reaction (PCR) amplification of telomerase products. PCR cycles were optimized to give as linear a signal as possible relative to telomerase products; 96-well streptavidin-coated PCR plates were used to isolate the preamplification telomerase products and to wash inhibitors away before the amplification step. The inhibitor removal step is critical to prevent false positives potentially caused by inhibition of Taq polymerase during amplification. Use of the streptavidin-coated PCR plate allows this step to be done much more rapidly than use of the liquid/liquid extraction adopted by others. We have demonstrated that this assay can correctly order the ability of four inhibitors to inhibit telomerase and reproduce within a factor of two the absolute IC(50) values determined by the more time-consuming direct assay. We have shown that the difference in IC(50) values determined in this assay versus the direct assay can be corrected for by using the standard curve appropriately. Using this method 96 compounds can be assessed in 3-5h.
Subject(s)
Drug Evaluation, Preclinical/methods , Enzyme Inhibitors/pharmacology , Polymerase Chain Reaction/methods , Telomerase/antagonists & inhibitors , Cell Extracts , DNA/analysis , DNA/metabolism , Fluorescent Dyes , Fluorometry , HeLa Cells , Humans , Inhibitory Concentration 50 , Organic Chemicals , Polymerase Chain Reaction/standards , Telomerase/metabolism , Time FactorsABSTRACT
The detection and eradication of pharyngeal Chlamydia trachomatis in patients with chlamydial uterine cervicitis (commercial sex workers and others) were investigated. Pharyngeal C. trachomatis was detected in 75.0% of the commercial sex workers and in 21.9% of the other subjects. All the pharyngeal C. trachomatis-positive patients had a past history of orogenital contact. Chlamydial infection was treated with clarithromycin for 7 or 14 days. The presence of C. trachomatis was determined by polymerase chain reaction (PCR) on days 8, 15, and 22 after completion of the treatment. In the 7-day treatment group, the eradication rate of pharyngeal C. trachomatis was 53.3%, 56.7%, and 60.0% on days 8, 15, and 22, respectively, after completion of the treatment, while the eradication rate of cervical C. trachomatis was 83.3%, 96.7%, and 100% on days 8, 15, and 22, respectively. The eradication rate of pharyngeal C. trachomatis in the 7-day treatment was significantly lower than that of cervical C. trachomatis, while there was no significant difference in the 14-day treatment. The eradication rate of pharyngeal C. trachomatis in the 14-day treatment was significantly higher than that in the 7-day treatment. Since the DNA of dead organisms may be detected because of high PCR sensitivity, appropriate therapeutic judgment by PCR could be done around day 22 after completion of the treatment.
Subject(s)
Anti-Bacterial Agents/pharmacology , Chlamydia Infections/drug therapy , Chlamydia trachomatis/drug effects , Clarithromycin/pharmacology , Adult , Anti-Bacterial Agents/administration & dosage , Anti-Bacterial Agents/therapeutic use , Cervix Uteri/microbiology , Chlamydia Infections/microbiology , Chlamydia trachomatis/genetics , Clarithromycin/administration & dosage , Clarithromycin/therapeutic use , Female , Humans , Microbial Sensitivity Tests , Pharynx/microbiology , Polymerase Chain Reaction/standards , Prospective Studies , Sensitivity and Specificity , Sex WorkABSTRACT
Previous studies had shown that recombinant DNA can be detected for several months in soil after the deposition of litter from transgenic (tg) plants. Here we show by PCR monitoring of field releases of tg sugar beet plants that during the growth of the plants the soil close to the plants and also plant material contains recombinant DNA, in the form of extracellular molecules. Surprisingly, the monitoring also revealed the presence of tg DNA in many field plots (30-70%) in which tg plants were never grown. These studies and the further monitoring during other tg sugar beet release experiments by PCR and a novel bioassay (measuring the transforming potential of recombinant DNA for Pseudomonas stutzeri) indicated that recombinant DNA was only detectable in the surface soil of field plots and their vicinity where flowering of the tg beet plants was allowed. Recombinant DNA was found in soil at a distance of 50 m from pollen-producing plants surrounded by a strip with hemp plants as a containment regime. It is concluded that recombinant DNA is deposited in soil during the growth of tg sugar beets and that a major mechanism of recombinant DNA spread in the environment is the dispersal of pollen which allows recombinant DNA to persist in the field plot for at least a year.
Subject(s)
Beta vulgaris/genetics , DNA, Recombinant/analysis , Environmental Monitoring/methods , Plants, Genetically Modified , Crops, Agricultural , Environmental Monitoring/standards , Pollen , Polymerase Chain Reaction/standards , Pseudomonas stutzeri/genetics , Soil/analysis , Transformation, GeneticABSTRACT
A DNA microarray to monitor the expression of bacterial metabolic genes within mixed microbial communities was designed and tested. Total RNA was extracted from pure and mixed cultures containing the 2,4-dichlorophenoxyacetic acid (2,4-D)-degrading bacterium Ralstonia eutropha JMP134, and the inducing agent 2,4-D. Induction of the 2,4-D catabolic genes present in this organism was readily detected 4, 7, and 24 h after the addition of 2,4-D. This strain was diluted into a constructed mixed microbial community derived from a laboratory scale sequencing batch reactor. Induction of two of five 2,4-D catabolic genes (tfdA and tfdC) from populations of JMP134 as low as 10(5) cells/ml was clearly detected against a background of 10(8) cells/ml. Induction of two others (tfdB and tfdE) was detected from populations of 10(6) cells/ml in the same background; however, the last gene, tfdF, showed no significant induction due to high variability. In another experiment, the induction of resin acid degradative genes was statistically detectable in sludge-fed pulp mill effluent exposed to dehydroabietic acid in batch experiments. We conclude that microarrays will be useful tools for the detection of bacterial gene expression in wastewaters and other complex systems.
Subject(s)
Bacteria/metabolism , Bioreactors , Gene Expression Profiling , Oligonucleotide Array Sequence Analysis , Waste Disposal, Fluid/methods , 2,4-Dichlorophenoxyacetic Acid/metabolism , Bacteria/genetics , Bacteria/growth & development , Bacterial Proteins/genetics , Bacterial Proteins/metabolism , Biodegradation, Environmental , Cupriavidus necator/genetics , Cupriavidus necator/growth & development , Cupriavidus necator/metabolism , DNA Probes , DNA, Complementary/genetics , DNA, Complementary/metabolism , Ecosystem , Industrial Waste , Oligonucleotide Array Sequence Analysis/methods , Oligonucleotide Array Sequence Analysis/standards , Paper , Polymerase Chain Reaction/methods , Polymerase Chain Reaction/standardsABSTRACT
To allow for pharmacokinetic studies in adjunction with the current clinical developments of the potent cytostatic anti-cancer drug rViscumin, a sandwich immuno-PCR (IPCR) assay was developed for the detection of rViscumin in blood plasma. The IPCR was carried out with a commercially available reagent kit, consisting of pre-assembled rViscumin-specific antibody-DNA conjugates as well as a specific competitor DNA fragment to be amplified by PCR. Various combinations of capture- and detection-antibodies were compared for performance in IPCR. Using the optimized assay, as few as 50 zeptomol (approx. 100 fg/ml) rViscumin (MW 57 kDa) was detectable in standardized human serum samples. The IPCR assay was very selective for rViscumin and in spiking experiments in proband plasma samples, signal recovery rates between 70% and 120% were obtained. The linear sensitivity range of the assay covered more than five orders of magnitude. Repeated measurements of rViscumin resulted in a mean standard deviation value of 14.2%.
Subject(s)
Plant Lectins/blood , Plant Preparations/blood , Plant Proteins , Polymerase Chain Reaction/methods , Toxins, Biological/blood , Animals , Antibody Specificity , Cross Reactions/immunology , Enzyme-Linked Immunosorbent Assay , Humans , Plant Lectins/genetics , Plant Lectins/immunology , Plant Preparations/immunology , Polymerase Chain Reaction/standards , Reproducibility of Results , Ribosome Inactivating Proteins, Type 2 , Sensitivity and Specificity , Toxins, Biological/genetics , Toxins, Biological/immunologyABSTRACT
Real time RT-PCR is the most sensitive method for quantitation of gene expression levels. The accuracy can be dependent on the mathematical model on which the quantitative methods are based. The generally accepted mathematical model assumes that amplification efficiencies are equal at the exponential phase of the reactions for the same amplicon. However, no methods are available to test the assumptions regarding amplification efficiency before one starts the real time PCR quantitation. Here we further develop and test the validity of a new mathematical model which dynamically fits real time PCR data with good correlation (R(2)=0.9995+/-0.002, n=50). The method is capable of measuring cycle-by-cycle PCR amplification efficiencies and demonstrates that these change dynamically. Validation of the method revealed the intrinsic relationship between the initial amount of gene transcript and kinetic parameters. A new quantitative method is proposed which represents a simple but accurate quantitative method.