Your search keyword '"Douglas Spencer"' showing total 9 results

1. Comparison of a novel HPV test with the Hybrid Capture II (hcII) and a reference PCR method shows high specificity and positive predictive value for 13 high-risk human papillomavirus infections

Author

Neralie Coulston, Cristina Baleriola, William D. Rawlinson, Douglas Spencer Millar, John R. Melki, Phillip Altman, and Nikolas Rismanto

Subjects

Polymerase Chain Reaction, Sensitivity and Specificity, law.invention, Predictive Value of Tests, law, Virology, medicine, Humans, Hpv test, Human papillomavirus, Papillomaviridae, Genotyping, Polymerase chain reaction, Cervical cancer, business.industry, Papillomavirus Infections, Hybrid capture, Australia, Nucleic Acid Hybridization, Cancer, medicine.disease, Predictive value, Infectious Diseases, Female, Reagent Kits, Diagnostic, business

Abstract

Background It is well established that human papillomavirus (HPV) infection is highly related to the development of precursor lesions of cervical cancer and uterine cancers. However, for a pre-cancerous lesion to develop, a persistent infection with a high-risk type HPV is necessary. The Digene Hybrid Capture II (hcII) assay is the only FDA approved method used in conjunction with cytology for HPV screening of women older than 30. The hcII has moderate sensitivity (64.7%) and is dependent on the cellular content of samples, rendering occasionally false positive and false negative results. Objective This study aims to evaluate the performance of a new HPV diagnostic kit (High-Risk HPV detection kit, manufactured by Human Genetic Signatures (HGS), Sydney, Australia). Methods The method under evaluation was assessed by comparing the results obtained from testing 834 cervical specimens with the HGS method and the Digene hcII method, using genotyping as the reference standard. Results Results of the study showed that the specificity and positive predictive value of the HGS High-Risk HPV detection test are significantly greater than those of the Digene hcII test. Overall the HGS HPV assay provides a more accurate system for the detection of high-risk HPV strains, with simpler technical use compared with PCR-sequencing methods.

Published

2008

2. Hypermethylation of the Inhibin α-Subunit Gene in Prostate Carcinoma

Author

Susan L. Clark, Gail P. Risbridger, Peter L. Molloy, Jacqueline F. Schmitt, Mark Frydenberg, Douglas Spencer Millar, Deon J. Venter, and John S. Pedersen

Subjects

Male, endocrine system, endocrine system diseases, Biopsy, Molecular Sequence Data, Loss of Heterozygosity, Biology, Polymerase Chain Reaction, Loss of heterozygosity, Mice, Prostate cancer, Endocrinology, Sequence Homology, Nucleic Acid, Gene expression, medicine, Animals, Humans, Inhibins, Promoter Regions, Genetic, Molecular Biology, Gene, Base Sequence, Prostatic Neoplasms, Promoter, General Medicine, DNA Methylation, medicine.disease, Molecular biology, Rats, CpG site, Chromosomes, Human, Pair 2, DNA methylation, Chromosomal region, Cancer research, Cattle, 5' Untranslated Regions, hormones, hormone substitutes, and hormone antagonists

Abstract

Inhibin is composed of an alpha- and a beta-subunit. Transgenic studies assigned a tumor-suppressive role to the inhibin alpha-subunit, and in human prostate cancer inhibin alpha-subunit gene expression was down-regulated. This study examined the inhibin alpha-subunit gene promoter and gene locus to determine whether promoter hypermethylation or LOH occurred in DNA from prostate cancer. The 5'-untranslated region of the human inhibin alpha-subunit gene was sequenced and shown to be highly homologous to the bovine, rat, and mouse inhibin alpha-subunit promoter sequences. A 135-bp region of the human promoter sequence that continued a cluster of CpG sites was analyzed for hypermethylation. Significant (P0.001) hypermethylation of the inhibin alpha-subunit gene promoter occurred in DNA from Gleason pattern 3, 4, and 5 carcinomas compared with nonmalignant tissue samples. A subset of the carcinomas with a cribriform pattern were unmethylated. LOH at 2q32-36, the chromosomal region harboring the inhibin alpha-subunit gene, was observed in 42% of prostate carcinomas. These data provide the first demonstration that promoter hypermethylation and LOH are associated with the inhibin alpha-subunit gene and gene locus in prostate cancer.

Published

2002

3. Quality control and optimized procedure of hybridization capture-PCR for the identification of Mycobacterium avium subsp. paratuberculosis in faeces

Author

R Whittington, I Marsh, and Douglas Spencer Millar

Subjects

Quality Control, Sheep Diseases, Paratuberculosis, Biology, Polymerase Chain Reaction, Microbiology, law.invention, Feces, law, medicine, Animals, Molecular Biology, In Situ Hybridization, Polymerase chain reaction, Southern blot, Sheep, Temperature, Nucleic acid sequence, DNA, Cell Biology, medicine.disease, biology.organism_classification, DNA extraction, Mycobacterium avium subsp. paratuberculosis, Flock, Camelids, New World, Mycobacterium avium, Mycobacterium

Abstract

Nucleic acid sequence capture techniques are used to improve both the sensitivity and specificity of PCR for the diagnosis of plant, animal and human diseases. Hybridization capture-PCR (HC-PCR) was first reported as a method for the detection of Mycobacterium avium subsp. paratuberculosis in 1995 and was successfully trialed on a small number of faecal samples from cattle with Johne's disease. A locally optimized HC-PCR method was evaluated on faeces from infected and non-infected animals. However, sample to sample cross contamination during the DNA purification step highlighted that the original format of the test was unsuitable for routine diagnostic use. Here, we report modifications and optimization of HC-PCR, particularly with respect to DNA purification from faeces, hybridization and capture steps. We also identified procedurally sensitive critical points in the test during capture and washing of magnetic beads. Southern blotting was omitted from the protocol to preserve specificity but this resulted in analytical sensitivity of 5000 organisms per 200 mg faecal sample. Nevertheless, HC-PCR detected M.paratuberculosis in pellets from infected sheep diluted at rates of up to 1 in 100 in normal faeces, suggesting that the technique should be evaluated further for low-cost diagnosis in flocks/herds using pooled samples.

Published

2000

4. Detailed methylation analysis of the glutathione S-transferase π (GSTP1) gene in prostate cancer

Author

Susan J. Clark, Douglas Spencer Millar, Kim K Ow, Pamela J. Russell, Peter L. Molloy, and Cheryl L. Paul

Subjects

Male, Cancer Research, Molecular Sequence Data, Biology, medicine.disease_cause, Polymerase Chain Reaction, GSTP1, Epigenetics of physical exercise, Tumor Cells, Cultured, Genetics, medicine, Humans, Cancer epigenetics, Promoter Regions, Genetic, Molecular Biology, Alleles, Glutathione Transferase, Base Sequence, Prostatic Neoplasms, Sequence Analysis, DNA, Methylation, DNA Methylation, Immunohistochemistry, Molecular biology, Isoenzymes, Differentially methylated regions, Glutathione S-Transferase pi, CpG site, DNA methylation, Cancer research, CpG Islands, Carcinogenesis

Abstract

Glutathione-S-Transferases (GSTs) comprise a family of isoenzymes that provide protection to mammalian cells against electrophilic metabolites of carcinogens and reactive oxygen species. Previous studies have shown that the CpG-rich promoter region of the pi-class gene GSTP1 is methylated at single restriction sites in the majority of prostate cancers. In order to understand the nature of abnormal methylation of the GSTP1 gene in prostate cancer we undertook a detailed analysis of methylation at 131 CpG sites spanning the promoter and body of the gene. Our results show that DNA methylation is not confined to specific CpG sites in the promoter region of the GSTP1 gene but is extensive throughout the CpG island in prostate cancer cells. Furthermore we found that both alleles are abnormally methylated in this region. In normal prostate tissue, the entire CpG island was unmethylated, but extensive methylation was found outside the island in the body of the gene. Loss of GSTP1 expression correlated with DNA methylation of the CpG island in both prostate cancer cell lines and cancer tissues whereas methylation outside the CpG island in normal prostate tissue appeared to have no effect on gene expression.

Published

1999

5. Detection and measurement of PCR bias in quantitative methylation analysis of bisulphite-treated DNA

Author

Douglas Spencer Millar, Clare Stirzaker, Peter M. Warnecke, Cheryl L. Paul, John R. Melki, and Susan J. Clark

Subjects

Biology, Polymerase Chain Reaction, Sensitivity and Specificity, DNA sequencing, Cell Line, law.invention, Cytosine, Mice, chemistry.chemical_compound, law, Primer dimer, Genetics, Animals, Humans, Sulfites, Genes, Retinoblastoma, Polymerase chain reaction, DNA Primers, Base Composition, Multiple displacement amplification, DNA, DNA Methylation, Molecular biology, genomic DNA, 5-Methylcytosine, chemistry, DNA methylation, Research Article, In silico PCR

Abstract

Methylation analysis of individual cytosines in genomic DNA can be determined quantitatively by bisulphite treatment and PCR amplification of the target DNA sequence, followed by restriction enzyme digestion or sequencing. Methylated and unmethylated molecules, however, have different sequences after bisulphite conversion. For some sequences this can result in bias during the PCR amplification leading to an inaccurate estimate of methylation. PCR bias is sequence dependent and often strand-specific. This study presents a simple method for detection and measurement of PCR bias for any set of primers, and investigates parameters for overcoming PCR bias.

Published

1997

6. Solid-Phase Hybridization Capture of Low-Abundance Target DNA Sequences: Application to the Polymerase Chain Reaction Detection of Mycobacterium paratuberculosis and Mycobacterium avium subsp. silvaticum

Author

Douglas Spencer Millar, S.J. Withey, J. Hermontaylor, J.G. Ford, and M.L.V. Tizard

Subjects

DNA, Bacterial, Molecular Sequence Data, Biophysics, Polymerase Chain Reaction, Sensitivity and Specificity, Biochemistry, DNA sequencing, law.invention, Feces, chemistry.chemical_compound, Crohn Disease, law, Animals, Humans, False Positive Reactions, Molecular Biology, Pathogen, Polymerase chain reaction, DNA Primers, Base Sequence, biology, Inverse polymerase chain reaction, Nucleic Acid Hybridization, Cell Biology, Amplicon, biology.organism_classification, Molecular biology, Intestines, Mycobacterium avium subsp. paratuberculosis, chemistry, Biotinylation, DNA Transposable Elements, Cattle, DNA, Mycobacterium avium, Mycobacterium

Abstract

Polymerase chain reaction (PCR) has been widely applied to the detection of microorganisms. Overall sensitivity of PCR tests may be substantially reduced due to a large excess of nontarget DNA and inhibitory substances in the sample. We used a 5'-biotinylated 513-bp probe from the 3' region of the IS 900 element specific for Mycobacterium paratuberculosis (Mptb) to capture target Mptb DNA from crude sample DNA extracts. Captured target DNA was separated using streptavidin-coated magnetic particles (Dynal). Since the IS 900 element shares homology over this region with IS 902 in Mycobacterium avium subsp. silvaticum (Mavs), target DNA from this other pathogen was also retained. Highly specific PCR for the detection of either organism directed to the 5' regions of IS 900 or IS 902 was then performed directly on the solid phase. Hybridization capture of target DNA using sequence adjacent to the desired specific PCR site applied to Mptb increased overall sensitivity of detection in tissue and fecal extracts 10- to 100-fold. False positives due to contamination artifact were substantially excluded since the capture probe did not retain amplicons from the detection PCR. Development of the method to involve covalent 5' immobilization of capture probes on heat-resistant polymers should, in the future, provide a simple system with broad potential applications.

Published

1995

7. A genomic sequencing protocol that yields a positive display of 5-methylcytosine residues in individual DNA strands

Author

Cheryl L. Paul, Fujiko Watt, Christina M. Collis, Peter L. Molloy, Geoffrey W. Grigg, Louise E. McDonald, Douglas Spencer Millar, and Marianne Frommer

Subjects

Molecular Sequence Data, Bisulfite sequencing, Biology, Methylation, Polymerase Chain Reaction, Cytosine, chemistry.chemical_compound, Heavy strand, Humans, Sulfites, Methylated DNA immunoprecipitation, Promoter Regions, Genetic, RNA-Directed DNA Methylation, Genetics, Multidisciplinary, Base Sequence, Kininogens, DNA, genomic DNA, 5-Methylcytosine, Oligodeoxyribonucleotides, chemistry, Biochemistry, DNA methylation, Illumina Methylation Assay, Research Article

Abstract

The modulation of DNA-protein interactions by methylation of protein-binding sites in DNA and the occurrence in genomic imprinting, X chromosome inactivation, and fragile X syndrome of different methylation patterns in DNA of different chromosomal origin have underlined the need to establish methylation patterns in individual strands of particular genomic sequences. We report a genomic sequencing method that provides positive identification of 5-methylcytosine residues and yields strand-specific sequences of individual molecules in genomic DNA. The method utilizes bisulfite-induced modification of genomic DNA, under conditions whereby cytosine is converted to uracil, but 5-methylcytosine remains nonreactive. The sequence under investigation is then amplified by PCR with two sets of strand-specific primers to yield a pair of fragments, one from each strand, in which all uracil and thymine residues have been amplified as thymine and only 5-methylcytosine residues have been amplified as cytosine. The PCR products can be sequenced directly to provide a strand-specific average sequence for the population of molecules or can be cloned and sequenced to provide methylation maps of single DNA molecules. We tested the method by defining the methylation status within single DNA strands of two closely spaced CpG dinucleotides in the promoter of the human kininogen gene. During the analysis, we encountered in sperm DNA an unusual methylation pattern, which suggests that the high methylation level of single-copy sequences in sperm may be locally modulated by binding of protein factors in germ-line cells.

Published

1992

8. Methylation sequencing from limiting DNA: embryonic, fixed, and microdissected cells

Author

Susan J. Clark, John R. Melki, Peter M. Warnecke, and Douglas Spencer Millar

Subjects

Paraffin Embedding, Embryo, Methylation, 3T3 Cells, Microtomy, Sequence Analysis, DNA, Biology, DNA Methylation, Embryonic stem cell, Molecular biology, Polymerase Chain Reaction, General Biochemistry, Genetics and Molecular Biology, Bisulfite, chemistry.chemical_compound, Mice, Blastocyst, chemistry, DNA methylation, Animals, Sulfites, Molecular Biology, Microdissection, DNA, Cells, Cultured, Laser capture microdissection

Abstract

It is frequently useful to determine the methylation state of samples containing limited amounts of DNA such as from embryos, or from fixed tissue samples in which DNA is degraded or difficult to isolate. By modification of the standard protocols for DNA preparation and bisulfite treatment, it is possible to obtain DNA methylation sequence data for such samples. We present methods for bisulfite treatment of embryos, fixed sections, and samples obtained by laser capture microdissection, and discuss the additional experimental considerations required when working with small numbers of cells or degraded DNA samples.

Published

2002

9. IS900 targets translation initiation signals in Mycobacterium avium subsp. paratuberculosis to facilitate expression of its hed gene

Author

Mark Loughlin, Jon Ford, Mark Tizard, John Hermon-Taylor, Douglas Spencer Millar, Timothy J. Doran, and Nazira Sumar

Subjects

Transposable element, Transcription, Genetic, Genetic Vectors, Paratuberculosis, Biology, Microbiology, Polymerase Chain Reaction, Start codon, Bacterial Proteins, Putative gene, medicine, RNA, Messenger, Insertion sequence, Peptide Chain Initiation, Translational, Gene, Gene Expression Regulation, Bacterial, medicine.disease, Molecular biology, Antibodies, Bacterial, Stop codon, Ribosomal binding site, RNA, Bacterial, Genes, Bacterial, Protein Biosynthesis, DNA Transposable Elements, Mycobacterium avium

Abstract

The Mycobacterium avium subsp. paratuberculosis (formerly Mycobacterium paratuberculosis) atypical insertion sequence, IS900, encodes a novel gene on the complementary strand to the putative transposase, p43. This gene requires a promoter, ribosome binding site (RBS) and termination codon to be acquired upon insertion into the M. avium subsp. paratuberculosis genome and hence is designated the hed (host expression-dependent) gene of IS900. Analysis of IS900 insertion sites suggests that this element targets translation initiation signals in M. avium subsp. paratuberculosis, specifically inserting between the RBS and start codon of a putative gene sequence. This aligns the hed initiation codon adjacent to a functional RBS and possibly downstream of an active promoter, driving expression of Hed protein. We have confirmed this unique targeting process by detecting expression of hed in M. avium subsp. paratuberculosis at the level of transcription by reverse transcription-PCR. Further, two Hed-specific antibodies detected Hed translation products in Western blots of protein extracts from M. avium subsp. paratuberculosis. A recombinant form of Hed expressed and purified from Escherichia coli will facilitate studies of IS900 transposition and will also be assessed as a diagnostic antigen for M. avium subsp. paratuberculosis disease. Implications of IS900 insertion in M. avium subsp. paratuberculosis pathogenicity are discussed.

Published

1997