Your search keyword '"Irvine Bruce"' showing total 9 results

1. Rapid and Precise Quantification of HIV-1 RNA in Plasma Using a Branched DNA Signal Amplification Assay

Author

Irvine Bruce, Carol Pachl, Paul Neuwald, Sue-Jane Fong, David G. Kern, Mickey S. Urdea, John Todd, Diana J. Besemer, Torange Yeghiazarian, Bradley S. Hoo, Robert Kokka, Patrick J. Sheridan, Janice A. Kolberg, and Michelle M. Stempien

Subjects

Branched DNA Signal Amplification Assay, Immunology, Acyclovir, DNA, Single-Stranded, Biology, Sensitivity and Specificity, Virus, chemistry.chemical_compound, Nucleic acid thermodynamics, Virology, HIV Seropositivity, BDNA test, medicine, Humans, Immunology and Allergy, Longitudinal Studies, medicine.diagnostic_test, Oligonucleotide, Gene Amplification, Nucleic Acid Hybridization, Reproducibility of Results, virus diseases, RNA, Genes, pol, Molecular biology, CD4 Lymphocyte Count, Didanosine, chemistry, Immunoassay, Disease Progression, HIV-1, RNA, Viral, Drug Therapy, Combination, Oligonucleotide Probes, Zidovudine, DNA

Abstract

The level of human immunodeficiency virus type 1 (HIV-1) RNA in human plasma has been quantitated directly with use of a solid-phase nucleic acid hybridization assay, based on branched DNA (bDNA) signal amplification technology with chemiluminescent detection. Signal amplification is accomplished by the incorporation of sites for 1,755 alkaline phosphatase-labeled probes per genome of HIV-1, after successive hybridization of target-specific oligonucleotides and bDNA amplifier molecules. The assay is performed in microwells, much like an immunoassay, and is amenable to routine laboratory use. Reproducibility and specificity studies indicated that the bDNA method was precise and showed no reactivity with seronegative donors. HIV-1 RNA levels were quantitated for 348 seropositive specimens, with a detection rate of 83% for those specimens from patients with < 500 CD4+ T-cell counts. Plasma RNA levels were found to change with disease stage, and in response to antiviral therapy. Quantitation of HIV-1 RNA in the plasma of HIV-1-infected patients, with use of the bDNA assay, may be a useful method for monitoring HIV-1 disease progression and therapeutic response.

Published

1995

2. Mechanical Disruption of Lysis-Resistant Bacterial Cells by Use of a Miniature, Low-Power, Disposable Device ▿†

Author

Gerard A. Cangelosi, Angelika Niemz, Irvine Bruce, Barbara Erwin, Kris M. Weigel, Ali Nadim, Peter E. Vandeventer, Jose Salazar, and Robert Doebler

Subjects

Microbiology (medical), DNA, Bacterial, Bacteriological Techniques, Chromatography, Lysis, biology, Microorganism, Sonication, Bacteriology, Bacillus subtilis, biology.organism_classification, Mycobacterium bovis, Microbiology, Bacteriolysis, Nucleic acid, Cell disruption, Humans, Bacteria, Mycobacterium

Abstract

Molecular detection of microorganisms requires microbial cell disruption to release nucleic acids. Sensitive detection of thick-walled microorganisms such as Bacillus spores and Mycobacterium cells typically necessitates mechanical disruption through bead beating or sonication, using benchtop instruments that require line power. Miniaturized, low-power, battery-operated devices are needed to facilitate mechanical pathogen disruption for nucleic acid testing at the point of care and in field settings. We assessed the lysis efficiency of a very small disposable bead blender called OmniLyse relative to the industry standard benchtop Biospec Mini-BeadBeater. The OmniLyse weighs approximately 3 g, at a size of approximately 1.1 cm 3 without the battery pack. Both instruments were used to mechanically lyse Bacillus subtilis spores and Mycobacterium bovis BCG cells. The relative lysis efficiency was assessed through real-time PCR. Cycle threshold ( C T ) values obtained at all microbial cell concentrations were similar between the two devices, indicating that the lysis efficiencies of the OmniLyse and the BioSpec Mini-BeadBeater were comparable. As an internal control, genomic DNA from a different organism was spiked at a constant concentration into each sample upstream of lysis. The C T values for PCR amplification of lysed samples using primers specific to this internal control were comparable between the two devices, indicating negligible PCR inhibition or other secondary effects. Overall, the OmniLyse device was found to effectively lyse tough-walled organisms in a very small, disposable, battery-operated format, which is expected to facilitate sensitive point-of-care nucleic acid testing.

Published

2011

3. At least five related, but distinct, hepatitis C viral genotypes exist

Author

Irvine Bruce, Tai-An Cha, Beall Eileen, G. Kuo, Janice A. Kolberg, Mickey S. Urdea, and D. Chien

Subjects

Genotype, Sequence analysis, Hepacivirus, Hepatitis C virus, Molecular Sequence Data, medicine.disease_cause, Polymerase Chain Reaction, Sequence Homology, Nucleic Acid, medicine, Humans, Amino Acid Sequence, Peptide sequence, Hepatitis, Genetics, Multidisciplinary, Base Sequence, biology, Nucleic acid sequence, Hepatitis C, biology.organism_classification, medicine.disease, Virology, Oligodeoxyribonucleotides, RNA, Viral, Oligonucleotide Probes, Software, Research Article

Abstract

Hepatitis C virus, the major causative agent of blood-borne non-A, non-B hepatitis in the world, has been the subject of considerable nucleic acid sequence analysis. Although all reported hepatitis C sequences from the United States have been represented by the prototype hepatitis C virus type 1 sequence, two groups of variant sequences have been reported in Japan. However, we have noted five distinct, but related, genotypes (I-V) throughout the world, based on detailed sequence determination and analysis of the first 1700 nucleotides and part of the nonstructural region 5 at the C terminus of the open reading frame. The nucleotide sequence for a large number of hepatitis C virus isolates spanning six continents was obtained by direct sequence analysis of PCR products after reverse transcription. Genotype was classified by using several distinct sequence motifs. We observed that most genotypes coexist in several geographic regions, including the United States, Japan, Germany, and Italy. So far, genotype V has been found only in South Africa. Interestingly, each distinct genotype seems to be maintained throughout the genome in the segments studied. These genotype distinctions should be considered when designing specific diagnostic tests, developing potential vaccines, and studying viral transmission.

Published

1992

4. A branched DNA signal amplification assay for quantification of nucleic acid targets below 100 molecules/ml

Author

Eric Fine, Chu-An Chang, Crystle L. K. Zayati, Diana Tyner, Jill Detmer, Irvine Bruce, David D. Ho, David Ahle, Mickey S. Urdea, Lu-Ping Shen, Janice A. Kolberg, Steve Bushnell, Mark L. Collins, and Thomas Horn

Subjects

Adenosine, Anti-HIV Agents, Branched DNA Signal Amplification Assay, HIV Infections, Cytidine, Biology, chemistry.chemical_compound, Nucleic acid thermodynamics, Genetics, BDNA test, Humans, Nucleotide, chemistry.chemical_classification, Nelfinavir, Guanosine, Oligonucleotide, HIV, Nucleic Acid Hybridization, DNA, Isoquinolines, Molecular biology, chemistry, Lamivudine, DNA, Viral, Nucleic acid, RNA, Viral, Drug Therapy, Combination, Sulfonic Acids, Viral load, Zidovudine, Research Article

Abstract

The branched DNA hybridization assay has been improved by the inclusion of the novel nucleotides, isoC and isoG, in the amplification sequences to prevent non-specific hybridization. The novel isoC, isoG-containing amplification sequences have no detectable interaction with any natural DNA sequence. The control of non-specific hybridization in turn permits increased signal amplification. Addition of a 14 site preamplifier was found to increase the signal/noise ratio 8-fold. A set of 74 oligonucleotide probes was designed to the consensus HIV POL sequence. The detection limit of this new HIV branched DNA amplifier assay was approximately 50 molecules/ml. The assay was used to measure viral load in 87 plasma samples of HIV- infected patients on triple drug therapy whose RNA titers were

Published

1997

5. Classification of hepatitis C virus into six major genotypes and a series of subtypes by phylogenetic analysis of the NS-5 region

Author

Janice A. Kolberg, Shiu-Wan Chan, Mickey S. Urdea, Irvine Bruce, Beall Eileen, F. McOmish, Tai-An Cha, P L Yap, Edward C. Holmes, and Peter Simmonds

Subjects

Genetics, biology, Phylogenetic tree, Base Sequence, Genotype, Hepacivirus, Hepatitis C virus, Molecular Sequence Data, Nucleic acid sequence, Viral Nonstructural Proteins, biology.organism_classification, medicine.disease_cause, Genome, Virology, Phylogenetics, Sequence Homology, Nucleic Acid, medicine, Humans, RNA, Viral, Gene, Phylogeny

Abstract

Hepatitis C virus (HCV) showed substantial nucleotide sequence diversity distributed throughout the viral genome, with many variants showing only 68 to 79% overall sequence similarity to one another. Phylogenetic analysis of nucleotide sequences derived from part of the gene encoding a non-structural protein (NS-5) has provided evidence for six major genotypes of HCV amongst a worldwide collection of 76 samples from HCV-infected blood donors and patients with chronic hepatitis. Many of these HCV types comprised a number of more closely related subtypes, leading to a current total of 11 genetically distinct viral populations. Phylogenetic analysis of other regions of the viral genome produced relationships between published sequences equivalent to those found in NS-5, apart from the more highly conserved 5' non-coding region in which only the six major HCV types, but not subtypes, could be differentiated. A new nomenclature for HCV variants is proposed in this communication that reflects the two-tiered nature of sequence differences between different viral isolates. The scheme classifies all known HCV variants to date, and describes criteria that would enable new variants to be assigned within the classification as they are discovered.

Published

1993

6. Comparison of hepatitis C virus markers in patients with NANB hepatitis

Author

Osami Inoue, Shigenobu Nagataki, Michiaki Koga, Irvine Bruce, Hiroshi Yatsuhashi, George Kuo, Kyousuke Mizuno, Beall Eileen, Mickey S. Urdea, Michitami Yano, Janice A. Kolberg, and Tai-An Cha

Subjects

Adult, Male, Hepatitis C virus, Hepacivirus, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, Virus, Liver disease, Antigen, Virology, medicine, Humans, Hepatitis Antibodies, Antigens, Viral, Aged, NS3, biology, Hepatitis C, Hepatitis C Antibodies, Middle Aged, medicine.disease, Real-time polymerase chain reaction, biology.protein, Female, Antibody, Hepatitis C Antigens, Biomarkers

Abstract

10 different HCV-specific assays and RT-PCR of the 5' untranslated region of HCV RNA were used to analyze sixty-four patients with chronic NANB liver disease. Po, CP-9 and C22 antigens are located in the putative core; C33c in the putative NS3; C100-3 in the putative NS3/4; KCL in the putative NS4/5 and C825 is located in the putative NS5. GOR protein is not part of the HCV genome, but antibodies to it appear to be present in response to a hepatitis C infection. Positive rates were 91% for Po, 89% for CP-9, 94% for C22, 97% for C33c, 88% for C100-3 (Ortho, EIA), 86% for C100-3 (Abbott, EIA), 84% for C100-3 (Ohtsuka, RIA), 88% for KCL, 59% for C825, 58% for GOR, and 83% for RT-PCR. There were 8 cases which were negative by all anti-C100 tests. 7 of these cases were positive by other anti-HCV markers and/or PCR suggesting the need for improved blood screening assays. There is a variation in the relative reactivity for different markers with different samples. Of the tests employed, anti C33c shows the highest positivity rate.

Published

1992

7. Use of a signature nucleotide sequence of hepatitis C virus for detection of viral RNA in human serum and plasma

Author

Jang Han, Q L Choo, Tai-An Cha, Irvine Bruce, Beall Eileen, Janice A. Kolberg, Michelle M. Stempien, M Yano, Michael Houghton, and G. Kuo

Subjects

Microbiology (medical), Hepatitis C virus, Molecular Sequence Data, Blood Donors, Hepacivirus, Biology, medicine.disease_cause, Polymerase Chain Reaction, Virus, law.invention, Japan, law, Complementary DNA, Sequence Homology, Nucleic Acid, medicine, Humans, Polymerase chain reaction, NS3, Base Sequence, Nucleic acid sequence, Virology, Molecular biology, Hepatitis C, Reverse transcriptase, United States, Reverse transcription polymerase chain reaction, RNA, Viral, Oligonucleotide Probes, Research Article

Abstract

The nucleic acid sequence of the putative 5'-untranslated (5PUT) region of hepatitis C virus (HCV), determined for samples obtained from a variety of geographic origins, was found to be over 98% conserved among all isolates. On the basis of this signature sequence for HCV, a viral RNA assay was developed by using cDNA synthesis with reverse transcriptase, followed by polymerase chain reaction (PCR). The new assay was compared with the Ortho-Chiron C100-3 HCV enzyme-linked immunosorbent assay to research radioimmunoassays for antibodies to the C33c and C22 HCV antigens and to the first reported set of HCV PCR primers designed from the NS3 domain. Plasma samples from 16 Japanese patients with non-A, non-B hepatitis (NANBH) and 16 immunoassay-positive blood donors from the United States were investigated. The 5PUT PCR primers were found to be superior to the NS3 primers in sensitivity and specificity (15 of 25 versus 3 of 25 of the C100 enzyme-linked immunosorbent assay-positive samples, respectively). Samples from two C100-negative patients with acute NANBH were found to react with the 5PUT primers but not with the NS3 primers. Also, two of three patients with chronic NANBH converted from reverse transcriptase PCR positive to negative after interferon treatment. Although the clinical significance of the presence or absence of HCV RNA in samples from patients is not fully understood, the use of probes and primers from the 5PUT region (as opposed to primers from other segments) should not lead to false-negative results due to nucleic acid sequence variations in viral isolates.

Published

1991

8. Sequence of a cDNA coding for human glutathione peroxidase confirms TGA encodes active site selenocysteine

Author

Irvine Bruce, Guy T. Mullenbach, Graeme I. Bell, Azita Tabrizi, and Robert A. Hallewell

Subjects

Biology, chemistry.chemical_compound, Selenium, Complementary DNA, Genetics, Humans, Amino Acid Sequence, Cysteine, Binding site, Gene, Peptide sequence, chemistry.chemical_classification, Glutathione Peroxidase, Binding Sites, Selenocysteine, Base Sequence, Glutathione peroxidase, Protein primary structure, Active site, DNA, Molecular biology, chemistry, Biochemistry, Genes, biology.protein

Published

1987

9. Short and long-term effects of interferon on serum markers of hepatitis C virus replication

Author

Irvine Bruce, Shigenobu Nagataki, Michiaki Koga, Osami Inoue, Tai-An Cha, Mickey S. Urdea, Janice A. Kolberg, Kaoru Inokuchi, Michelle M. Stempien, Hiroshi Yatsuhashi, and Michitami Yano

Subjects

Male, Time Factors, medicine.medical_treatment, Hepatitis C virus, Radioimmunoassay, Hepacivirus, medicine.disease_cause, Virus Replication, Polymerase Chain Reaction, Virus, Serology, Interferon, medicine, Humans, Hepatitis Antibodies, Hepatitis, Chronic, Chemotherapy, Hepatology, business.industry, Gastroenterology, virus diseases, Interferon-alpha, Alanine Transaminase, Hepatitis C, Hepatitis C Antibodies, Middle Aged, medicine.disease, digestive system diseases, Cytokine, Immunology, RNA, Viral, Female, Viral disease, business, medicine.drug

Abstract

Hepatitis C virus RNA (HCV-RNA) and serological markers of HCV infection were measured in 30 patients with chronic hepatitis C who had been treated with interferon (IFN). Patients were classified into four groups according to serum alanine aminotransferase (ALT) levels after treatment. These were: as complete responders (CR); partial responders (PR); transient responders (TR); and non-responders (NR). In all 11 patients in the CR group, HCV-RNA disappeared from serum for at least 24 months and anti-c100-3 decreased progressively during this time. In the PR group, four of five patients were positive for HCV-RNA in spite of the improvement of ALT levels and decline of anti-c100-3. In the TR and NR groups, HCV-RNA disappeared transiently or remained persistently positive. The results indicate that IFN-mediated improvement of ALT and decrease of anti-HCV (anti-c100-3) were not always related to the disappearance of HCV-RNA from serum. On the other hand, sustained disappearance of HCV-RNA from serum was demonstrated in the patients who did not have post-treatment ALT relapse. This indicates that IFN can eradicate HCV from serum in some patients and provide a clinical remission of chronic hepatitis C.