Your search keyword '"Christopher P. Kolbert"' showing total 54 results

1. Correction: Multi-Platform Analysis of MicroRNA Expression Measurements in RNA from Fresh Frozen and FFPE Tissues.

Author

Christopher P. Kolbert, Rod M. Feddersen, Fariborz Rakhshan, Diane E. Grill, Gyorgy Simon, Sumit Middha, Jin Sung Jang, Vernadette Simon, Debra A. Schultz, Michael Zschunke, Wilma Lingle, Jennifer M. Carr, E. Aubrey Thompson, Ann L. Oberg, Bruce W. Eckloff, Eric D. Wieben, Peter Li, Ping Yang, and Jin Jen

Subjects

Medicine, Science

Published

2014

2. Supplementary Table 2 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 87KB, Differentially Expressed Genes by miR-708 Status in Never-Smoker Lung Adenocarcinoma.

Published

2023

3. Supplementary Table 3 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 58KB, Potential Target Genes of miR-708.

Published

2023

4. Data from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

Purpose: miRNA plays an important role in human disease and cancer. We seek to investigate the expression status, clinical relevance, and functional role of miRNA in non–small cell lung cancer.Experimental Design: We conducted miRNA expression profiling in matched lung adenocarcinoma and uninvolved lung using 56 pairs of fresh-frozen (FF) and 47 pairs of formalin-fixed, paraffin-embedded (FFPE) samples from never smokers. The most differentially expressed miRNA genes were evaluated by Cox analysis and log-rank test. Among the best candidate, miR-708 was further examined for differential expression in two independent cohorts. Functional significance of miR-708 expression in lung cancer was examined by identifying its candidate mRNA target and through manipulating its expression levels in cultured cells.Results: Among the 20 miRNAs most differentially expressed between tested tumor and normal samples, high expression level of miR-708 in the tumors was most strongly associated with an increased risk of death after adjustments for all clinically significant factors including age, sex, and tumor stage (FF cohort: HR, 1.90; 95% CI, 1.08–3.35; P = 0.025 and FFPE cohort: HR, 1.93; 95% CI, 1.02–3.63; P = 0.042). The transcript for TMEM88 gene has a miR-708 binding site in its 3′ UTR and was significantly reduced in tumors high of miR-708. Forced miR-708 expression reduced TMEM88 transcript levels and increased the rate of cell proliferation, invasion, and migration in culture.Conclusions: miRNA-708 acts as an oncogene contributing to tumor growth and disease progression by directly downregulating TMEM88, a negative regulator of the Wnt signaling pathway in lung cancer. Clin Cancer Res; 18(13); 3658–67. ©2012 AACR.

Published

2023

5. Supplementary Figure 3 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 154KB, TMEM88 is a putative target of miR-708 by MicroCosm database. The target site of miR-708 is located in the 3'UTR, 286 to 309 bases from downstream of the stop codon sequence of TMEM88. Asterisks indicate the binding site.

Published

2023

6. Supplementary Figure 1 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 147KB, Validation of miR-708 Overexpression by Real-Time qPCR in Lung Squamous cell carcinoma. Non-paired mostly smoker Squamous cell carcinomas and normal FFPE tissues from the National Cancer Institute cohort were examined. Sample numbers (n) and tissue types are indicated on each graph. P values are as shown by unpaired 2-tailed t test.

Published

2023

7. Supplementary Figure 2 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 90KB, Endogenous expression level of miR-708 in various cell lines. Real-time quantitative polymerase chain reaction analyses were performed as described in the "Methods" section.

Published

2023

8. Supplementary Table 1 from Increased miR-708 Expression in NSCLC and Its Association with Poor Survival in Lung Adenocarcinoma from Never Smokers

Author

Jin Jen, Ping Yang, Curtis C. Harris, Jae Yong Park, Ruth Lupu, Christopher P. Kolbert, Debra A. Schultz, Fariborz Rakhshan, Cheol-Hong Park, Hui Tang, Marie Christine Aubry, Zhifu Sun, Hyo-Sung Jeon, and Jin Sung Jang

Abstract

PDF file, 69KB, Clinical Information of the three lung adenocarcinoma Cohorts.

Published

2023

9. Brain expression genome-wide association study (eGWAS) identifies human disease-associated variants.

Author

Fanggeng Zou, High Seng Chai, Curtis S Younkin, Mariet Allen, Julia Crook, V Shane Pankratz, Minerva M Carrasquillo, Christopher N Rowley, Asha A Nair, Sumit Middha, Sooraj Maharjan, Thuy Nguyen, Li Ma, Kimberly G Malphrus, Ryan Palusak, Sarah Lincoln, Gina Bisceglio, Constantin Georgescu, Naomi Kouri, Christopher P Kolbert, Jin Jen, Jonathan L Haines, Richard Mayeux, Margaret A Pericak-Vance, Lindsay A Farrer, Gerard D Schellenberg, Alzheimer's Disease Genetics Consortium, Ronald C Petersen, Neill R Graff-Radford, Dennis W Dickson, Steven G Younkin, and Nilüfer Ertekin-Taner

Subjects

Genetics, QH426-470

Abstract

Genetic variants that modify brain gene expression may also influence risk for human diseases. We measured expression levels of 24,526 transcripts in brain samples from the cerebellum and temporal cortex of autopsied subjects with Alzheimer's disease (AD, cerebellar n=197, temporal cortex n=202) and with other brain pathologies (non-AD, cerebellar n=177, temporal cortex n=197). We conducted an expression genome-wide association study (eGWAS) using 213,528 cisSNPs within ± 100 kb of the tested transcripts. We identified 2,980 cerebellar cisSNP/transcript level associations (2,596 unique cisSNPs) significant in both ADs and non-ADs (q

Published

2012

10. DNA methylation and RNA expression profiles in lung adenocarcinomas of never-smokers

Author

Julie M. Cunningham, Aaron S. Mansfield, Jin Jen, Christopher P. Kolbert, Liang Wang, Zhifu Sun, and Ping Yang

Subjects

Male, Cancer Research, Lung Neoplasms, Adenocarcinoma of Lung, Adenocarcinoma, Biology, Article, Epigenesis, Genetic, Gene expression, Genetics, medicine, Humans, RNA, Messenger, Epigenetics, Promoter Regions, Genetic, Lung cancer, Molecular Biology, Aged, Principal Component Analysis, Smoking, Methylation, DNA Methylation, Middle Aged, medicine.disease, Molecular biology, Differentially methylated regions, CpG site, DNA methylation, Cancer research, Homeobox, CpG Islands, Female

Abstract

Lung cancer occurs in never-smokers. Epigenetic changes in lung cancer potentially represent important diagnostic, prognostic, and therapeutic targets. We compared DNA methylation profiles of 28 adenocarcinomas of the lungs of never-smokers with paired adjacent nonmalignant lung tissue. We correlated differential methylation changes with gene expression changes from the same 28 sample pairs. Using principal component analysis, we observed a distinct separation in methylation profiles between tumor and adjacent nonmalignant lung tissue. Tumors were generally hypomethylated compared with adjacent nonmalignant tissue. Of 1,906 CpG sites differentially methylated between tumor and nonmalignant tissue, 1,198 were within classically defined CpG islands where tumors were hypermethylated compared with nonmalignant tissue. A total of 708 sites were outside CpG islands where tumors were hypomethylated compared with nonmalignant tissue. There were significant differences in expression of 351 genes (23%) of the 1,522 genes matched to the differentially methylated CpG sites. Genes that were not significantly differentially expressed and were hypermethylated within CpG sites were enriched for homeobox genes. These results suggest that the methylation profiles of lung adenocarcinomas of never-smokers and adjacent nonmalignant lung tissue are significantly different. Despite the differential methylation of homeobox genes, no significant changes in expression of these genes were detected.

Published

2015

11. Intra-articular decorin influences the fibrosis genetic expression profile in a rabbit model of joint contracture

Author

Mark E. Morrey, Diane E. Grill, Matthew P. Abdel, Christopher P. Kolbert, Joaquin Sanchez-Sotelo, Jonathan D. Barlow, Scott P. Steinmann, B. F. Morrey, and Kai Nan An

Subjects

musculoskeletal diseases, medicine.medical_specialty, Pathology, Decorin, Rabbit Model, Genetic Expression, Fibrosis, Internal medicine, Gene expression, medicine, Orthopedics and Sports Medicine, Knee, Joint Contracture, Arthrofibrosis, Muscle contracture, Flexion contracture, business.industry, medicine.disease, Joint Contractures, Endocrinology, Surgery, Contracture, medicine.symptom, business

Abstract

Objectives The goal of this study was to determine whether intra-articular administration of the potentially anti-fibrotic agent decorin influences the expression of genes involved in the fibrotic cascade, and ultimately leads to less contracture, in an animal model. Methods A total of 18 rabbits underwent an operation on their right knees to form contractures. Six limbs in group 1 received four intra-articular injections of decorin; six limbs in group 2 received four intra-articular injections of bovine serum albumin (BSA) over eight days; six limbs in group 3 received no injections. The contracted limbs of rabbits in group 1 were biomechanically and genetically compared with the contracted limbs of rabbits in groups 2 and 3, with the use of a calibrated joint measuring device and custom microarray, respectively. Results There was no statistical difference in the flexion contracture angles between those limbs that received intra-articular decorin versus those that received intra-articular BSA (66° vs 69°; p = 0.41). Likewise, there was no statistical difference between those limbs that received intra-articular decorin versus those who had no injection (66° vs 72°; p = 0.27). When compared with BSA, decorin led to a statistically significant increase in the mRNA expression of 12 genes (p < 0.01). In addition, there was a statistical change in the mRNA expression of three genes, when compared with those without injection. Conclusions In this model, when administered intra-articularly at eight weeks, 2 mg of decorin had no significant effect on joint contractures. However, our genetic analysis revealed a significant alteration in several fibrotic genes. Cite this article: Bone Joint Res 2014;3:82–8.

Published

2014

12. Serodiagnosis of Human Granulocytic Ehrlichiosis by Using Novel Combinations of Immunoreactive Recombinant Proteins

Author

David H. Persing, Patricia D. Mcneill, Eric P. Hofmeister, Darin R. Benson, Steven G. Reed, Elizabeth S. Bruinsma, Raodoh Mohamath, Lisa D. Reynolds, Christopher P. Kolbert, Raymond L. Houghton, and Michael J. Lodes

Subjects

Microbiology (medical), Blotting, Western, Molecular Sequence Data, Ehrlichia, Enzyme-Linked Immunosorbent Assay, Biology, law.invention, Serology, Conserved sequence, Bacterial Proteins, Antigen, law, Humans, Direct repeat, Amino Acid Sequence, ORFS, Antigens, Bacterial, Base Sequence, Immunodominant Epitopes, Ehrlichiosis, Bacteriology, Sequence Analysis, DNA, biology.organism_classification, Antibodies, Bacterial, Fusion protein, Virology, Molecular biology, Recombinant Proteins, Recombinant DNA, Granulocytes

Abstract

A panel of seven recombinant antigens, derived from Ehrlichia phagocytophila (the agent of human granulocytic ehrlichiosis), was evaluated by class-specific enzyme-linked immunosorbent assays (ELISAs) for utility in the diagnosis of the infection. Fourteen genomic fragments, obtained by serologic expression screening, contained open reading frames (ORFs) encoding 16 immunodominant antigens. Eleven of these antigens were members of the major surface protein (MSP) multigene family. Alignment of their predicted protein sequences revealed a pattern of conserved sequences, which contained short direct repeats, flanking a variable region. In addition, two genomic clones contained two and three MSP ORFs, respectively, indicating that these genes are clustered in tandem copies. The implications for this pattern of both genomic and protein arrangements in antigenic variations of MSPs and in their utilities in a diagnostic assay are discussed. In addition to two MSP recombinant antigens (rHGE-1 and -3) and a fusion protein of these antigens (rErf-1), five further recombinants were evaluated by ELISA. Two of these antigens (rHGE-14 and -15) were novel, while a third (rHGE-2), with no known function, has been described. The final two recombinant antigens (rHGE-9 and -17) represent overlapping segments of the ankyrin gene ( ank ). The addition of rHGE-9 ELISA data resulted in the detection of 78% (21 of 27) of acute-phase sera. When serologic data for all recombinants are combined, 96.2% (26 of 27) of convalescent-phase patient serum samples and 85.2% (23 of 27) of acute-phase patient serum samples are detected, indicating the potential of these antigens for use in the development of a rapid serologic assay for the detection of E. phagocytophila infection.

Published

2001

13. Characterization of culture-derived spiral bacteria by 16S ribosomal RNA gene sequence analysis

Author

Christopher P. Kolbert, Randall T. Hayden, Marlene K. Hopkins, and David H. Persing

Subjects

Adult, DNA, Bacterial, Male, Microbiology (medical), Sequence analysis, Molecular Sequence Data, DNA, Ribosomal, Campylobacter fetus, Borrelia burgdorferi Group, RNA, Ribosomal, 16S, Humans, Gene, Ribosomal DNA, Genetics, Bacteria, Base Sequence, Sequence Homology, Amino Acid, biology, Sequence Analysis, RNA, Gene Amplification, Nucleic acid sequence, RNA, General Medicine, Middle Aged, Ribosomal RNA, 16S ribosomal RNA, biology.organism_classification, Infectious Diseases, Female

Abstract

Broad range amplification and sequence analysis of the 16S ribosomal RNA gene was used to identify three spiral-form organisms. The agents were identified as Campylobacter fetus, "Flexispira rappini", and Borrelia burgdorferi, respectively, using either proprietary or public sequence databases. In each case, the rDNA sequence showed 99-100% homology with known sequence data. Sequence-based analysis for each isolate required only 2-3 days, whereas traditional means of identification took 8-12 days to complete. The identification of spirochetes and vibrio-like agents from human clinical samples is often time consuming and results may be difficult to interpret, sometimes due to atypical phenotypic characteristics. Analysis of 16S rDNA or other molecular targets may provide a way to accurately and rapidly characterize isolates that are recalcitrant to speciation.

Published

2001

14. Bordetella holmesii–Like Organisms Associated with Septicemia, Endocarditis, and Respiratory Failure

Author

Yi-Wei Tang, Paul A. Hartley, Perry J. Severance, David H. Persing, Christopher P. Kolbert, and Marlene K. Hopkins

Subjects

Adult, Male, Microbiology (medical), Fastidious organism, Adolescent, Bordetella, Bacillus, Microbiology, RNA, Ribosomal, 16S, Sepsis, medicine, Humans, Endocarditis, Pathogen, Bordetella holmesii, biology, Endocarditis, Bacterial, biology.organism_classification, medicine.disease, RNA, Bacterial, Infectious Diseases, Sputum, Female, medicine.symptom, Respiratory Insufficiency, Bacteria

Abstract

We recovered an unusual bacterial strain from blood or sputum of three patients with septicemia, endocarditis, and/or respiratory failure. The three isolates were thin, curved, gram-negative, light brown, pigment-producing bacilli with variable catalase activity. They were asaccharolytic, oxidase-negative, nonmotile, and fastidious. Identification was not possible on the basis of these characteristics alone or in combination with cellular fatty acid profiles. Nucleic acid amplification and sequence analysis of the 16S rRNA gene revealed that all three isolates were identical and most closely related to the emerging pathogen Bordetella holmesii, diverging from the published sequence at three nucleotide positions (99.8% similarity). Isolation of a B. holmesii-like pathogen from sputum suggests that, in addition to producing septicemia, the organism may inhabit the respiratory tract like other Bordetella species.

Published

1998

15. Correction: Multi-Platform Analysis of MicroRNA Expression Measurements in RNA from Fresh Frozen and FFPE Tissues

Author

Michael A. Zschunke, Peter W. Li, E. Aubrey Thompson, Ping Yang, Eric D. Wieben, Vernadette Simon, Fariborz Rakhshan, Christopher P. Kolbert, Diane E. Grill, Jennifer M. Carr, Jin Sung Jang, Debra A. Schultz, Sumit Middha, György J. Simon, Rod M. Feddersen, Bruce W. Eckloff, Wilma L. Lingle, Ann L. Oberg, and Jin Jen

Subjects

Multidisciplinary, Science, lcsh:R, RNA, Correction, lcsh:Medicine, Biology, Cell biology, microRNA, Fresh frozen, Medicine, lcsh:Q, lcsh:Science, Multi platform

Published

2014

16. Borrelia burgdorferi enzyme-linked immunosorbent assay for discrimination of OspA vaccination from spirochete infection

Author

Christopher P. Kolbert, Y Q Zhang, Dane A. Mathiesen, David H. Persing, E Fikrig, R T Schoen, and J Anderson

Subjects

Microbiology (medical), Lipoproteins, Enzyme-Linked Immunosorbent Assay, Spirochaetaceae, complex mixtures, Lyme disease, Borrelia burgdorferi Group, medicine, Humans, Borrelia burgdorferi, Lyme Disease, Vaccines, Synthetic, biology, medicine.diagnostic_test, Vaccine trial, bacterial infections and mycoses, biology.organism_classification, medicine.disease, Virology, Vaccination, Bacterial vaccine, Immunoassay, Antigens, Surface, Bacterial Vaccines, Immunology, bacteria, Vaccine failure, Research Article, Bacterial Outer Membrane Proteins

Abstract

Recombinant Lyme disease vaccines based on purified preparations of outer surface protein A (OspA) have been shown to be effective in preventing transmission of Borrelia burgdorferi in experimental animal models and are now being tested in humans. Since the most widely used screening tests for Lyme disease are based on a whole-cell sonicate of B. burgdorferi, serologic false positivity in vaccinated persons could result from reactivity to OspA within the antigen preparation. In order to avoid serologic false positivity in vaccinated subjects, we developed an immunoassay based on a low-passage-number, naturally occurring variant of B. burgdorferi which lacks the plasmid encoding OspA and OspB. The use of an antigen preparation derived from this organism provided sensitive and specific detection of B. burgdorferi seropositivity in experimental animals and in human Lyme disease cases. The OspA-B-negative enzyme-linked immunosorbent assay (ELISA) also appeared to be capable of discriminating the vaccinated state from vaccine failure and natural infection in experimental animals. Sera from human subjects participating in a vaccine trial gave false-positive results with an ELISA based on an OspA-containing strain, but no such reactivity was observed when the OspA-negative ELISA was used. We conclude that low-passage-number OspA-B-negative isolates in immunoassays may become useful for the immunologic discrimination of the vaccinated state, natural infection, and vaccine failure.

Published

1997

17. O5–01–05: Haplotypes at the MAPT locus associate with risk for LOAD and brain gene expression

Author

Neill R. Graff-Radford, Jin Jen, Li Ma, Thuy Nguyen, Ronald C. Petersen, High Seng Chai, Minerva M. Carrasquillo, Kimberly G. Malphrus, Zachary S. Quicksall, Sarah Lincoln, Steven G. Younkin, Mariet Allen, Vernon S. Pankratz, Fanggeng Zou, Gina Bisceglio, Michaela Kachadoorian, Curtis S. Younkin, Dennis W. Dickson, Christopher P. Kolbert, Julia E. Crook, Nilufer Ertekin-Taner, and Siddarth Krishnan

Subjects

Genetics, Psychiatry and Mental health, Cellular and Molecular Neuroscience, Developmental Neuroscience, Epidemiology, Health Policy, Haplotype, Gene expression, Locus (genetics), Neurology (clinical), Geriatrics and Gerontology, Biology

Published

2013

18. Multi-platform analysis of microRNA expression measurements in RNA from fresh frozen and FFPE tissues

Author

Debra A. Schultz, Peter W. Li, Sumit Middha, Vernadette Simon, Jennifer M. Carr, E. Aubrey Thompson, Christopher P. Kolbert, Fariborz Rakhshan, Eric D. Wieben, Rod M. Feddersen, Wilma L. Lingle, Jin Jen, Jin Sung Jang, Ann L. Oberg, Michael A. Zschunke, Bruce W. Eckloff, György J. Simon, Diane E. Grill, and Ping Yang

Subjects

Tissue Fixation, Microarrays, Gene Expression, lcsh:Medicine, Computational biology, Biology, Biochemistry, DNA sequencing, Cell Line, Molecular Genetics, Genome Analysis Tools, Formaldehyde, Nucleic Acids, microRNA, Gene expression, Humans, Genome Sequencing, lcsh:Science, Gene, Oligonucleotide Array Sequence Analysis, Genetics, Multidisciplinary, Paraffin Embedding, Gene Expression Profiling, lcsh:R, RNA, High-Throughput Nucleotide Sequencing, Reproducibility of Results, Computational Biology, Genomics, Comparative Genomics, Gene expression profiling, MicroRNAs, lcsh:Q, RNA extraction, DNA microarray, Genome Expression Analysis, Sequence Analysis, Research Article, Biotechnology

Abstract

MicroRNAs play a role in regulating diverse biological processes and have considerable utility as molecular markers for diagnosis and monitoring of human disease. Several technologies are available commercially for measuring microRNA expression. However, cross-platform comparisons do not necessarily correlate well, making it difficult to determine which platform most closely represents the true microRNA expression level in a tissue. To address this issue, we have analyzed RNA derived from cell lines, as well as fresh frozen and formalin-fixed paraffin embedded tissues, using Affymetrix, Agilent, and Illumina microRNA arrays, NanoString counting, and Illumina Next Generation Sequencing. We compared the performance within- and between the different platforms, and then verified these results with those of quantitative PCR data. Our results demonstrate that the within-platform reproducibility for each method is consistently high and although the gene expression profiles from each platform show unique traits, comparison of genes that were commonly detectable showed that detection of microRNA transcripts was similar across multiple platforms.

Published

2013

19. O3‐11‐03: Genetic association of variants with late‐onset Alzheimer's disease risk and brain gene expression

Author

Sumit Middha, Sarah Lincoln, Steven G. Younkin, Neill R. Graff-Radford, Thuy Nguyen, Fanggeng Zou, Lindsay A. Farrer, Ronald C. Petersen, High Seng Chai, Mariet Allen, Jin Jen, Nilufer Ertekin-Taner, Dennis W. Dickson, Christopher P. Kolbert, Julia E. Crook, Ryan Palusak, Christopher Rowley, Jonathan L. Haines, Margaret A. Pericak-Vance, Sooraj Maharjan, Kimberly G. Malphrus, Gina Bisceglio, Vernon S. Pankratz, Curtis S. Younkin, Gerard D. Schellenberg, Li Ma, Minerva M. Carrasquillo, Richard Mayeux, Constantin Georgescu, and Asha Nair

Subjects

Genetics, Epidemiology, Health Policy, Late onset, Genome-wide association study, Biology, Psychiatry and Mental health, Cellular and Molecular Neuroscience, Developmental Neuroscience, Gene expression, Disease risk, Neurology (clinical), Geriatrics and Gerontology, Common disease-common variant, Genetic association

Published

2012

20. P1‐201: Identification of human disease‐associated variants in a brain expression genome‐wide association study (eGWAS)

Author

Nilufer Ertekin-Taner, Christopher Rowley, Sarah Lincoln, Jin Jen, Vernon S. Pankratz, Li Ma, Thuy Nguyen, Constantin Georgescu, Neill R. Graff-Radford, Asha Nair, Mariet Allen, Sooraj Maharjan, Kimberly G. Malphrus, Naomi Kouri, Curtis S. Younkin, Gina Bisceglio, Sumit Middha, Minerva M. Carrasquillo, Christopher P. Kolbert, Julia E. Crook, Fanggeng Zou, Dennis W. Dickson, Steven G. Younkin, Ryan Palusak, Ronald C. Petersen, and High Seng Chai

Subjects

Psychiatry and Mental health, Cellular and Molecular Neuroscience, Brain expression, Human disease, Developmental Neuroscience, Epidemiology, Health Policy, Identification (biology), Genome-wide association study, Neurology (clinical), Computational biology, Geriatrics and Gerontology, Biology

Published

2012

21. O5‐03‐03: Genetic association of progressive supranuclear palsy (PSP) risk loci variants with brain gene expression and neuropathology endophenotypes

Author

Christopher P. Kolbert, Julia E. Crook, Ronald C. Petersen, Thuy Nguyen, Vernon S. Pankratz, Sarah Lincoln, Gina Bisceglio, High Seng Chai, Fanggeng Zou, Curtis S. Younkin, Li Ma, Mariet Allen, Sooraj Maharjan, Jin Jen, Gerard D. Schellenberg, Melissa E. Murray, Daniel J. Serie, Constantin Georgescu, Asha Nair, Ryan Palusak, Nilufer Ertekin-Taner, Kimberly G. Malphrus, Neill R. Graff-Radford, Dennis W. Dickson, Minerva M. Carrasquillo, Christopher Rowley, Naomi Kouri, Steven G. Younkin, and Sumit Middha

Subjects

Genetics, Epidemiology, Health Policy, Neuropathology, Biology, medicine.disease, Progressive supranuclear palsy, Psychiatry and Mental health, Cellular and Molecular Neuroscience, Developmental Neuroscience, Endophenotype, Gene expression, medicine, Neurology (clinical), Geriatrics and Gerontology, Genetic association

Published

2012

22. Novel late-onset Alzheimer disease loci variants associate with brain gene expression

Author

Mariet, Allen, Fanggeng, Zou, High Seng, Chai, Curtis S, Younkin, Julia, Crook, V Shane, Pankratz, Minerva M, Carrasquillo, Christopher N, Rowley, Asha A, Nair, Sumit, Middha, Sooraj, Maharjan, Thuy, Nguyen, Li, Ma, Kimberly G, Malphrus, Ryan, Palusak, Sarah, Lincoln, Gina, Bisceglio, Constantin, Georgescu, Debra, Schultz, Fariborz, Rakhshan, Christopher P, Kolbert, Jin, Jen, Jonathan L, Haines, Richard, Mayeux, Margaret A, Pericak-Vance, Lindsay A, Farrer, Gerard D, Schellenberg, Ronald C, Petersen, Neill R, Graff-Radford, Dennis W, Dickson, Steven G, Younkin, Nilüfer, Ertekin-Taner, Liana G, Apostolova, Steven E, Arnold, Clinton T, Baldwin, Robert, Barber, Michael M, Barmada, Thomas, Beach, Gary W, Beecham, Duane, Beekly, David A, Bennett, Eileen H, Bigio, Thomas D, Bird, Deborah, Blacker, Bradley F, Boeve, James D, Bowen, Adam, Boxer, James R, Burke, Jacqueline, Buros, Joseph D, Buxbaum, Nigel J, Cairns, Laura B, Cantwell, Chuanhai, Cao, Chris S, Carlson, Regina M, Carney, Steven L, Carroll, Helena C, Chui, David G, Clark, Jason, Corneveaux, Carl W, Cotman, Paul K, Crane, Carlos, Cruchaga, Jeffrey L, Cummings, Philip L, De Jager, Charles, DeCarli, Steven T, DeKosky, F Yesim, Demirci, Ramon, Diaz-Arrastia, Malcolm, Dick, Beth A, Dombroski, Ranjan, Duara, William D, Ellis, Denis, Evans, Kelley M, Faber, Kenneth B, Fallon, Martin R, Farlow, Steven, Ferris, Tatiana M, Foroud, Matthew, Frosch, Douglas R, Galasko, Paul J, Gallins, Mary, Ganguli, Marla, Gearing, Daniel H, Geschwind, Bernardino, Ghetti, John R, Gilbert, Sid, Gilman, Bruno, Giordani, Jonathan D, Glass, Alison M, Goate, Robert C, Green, John H, Growdon, Hakon, Hakonarson, Ronald L, Hamilton, John, Hardy, Lindy E, Harrell, Elizabeth, Head, Lawrence S, Honig, Matthew J, Huentelman, Christine M, Hulette, Bradley T, Hyman, Gail P, Jarvik, Gregory A, Jicha, Lee-Way, Jin, Gyungah, Jun, M Ilyas, Kamboh, Jason, Karlawish, Anna, Karydas, John S K, Kauwe, Jeffrey A, Kaye, Nancy, Kennedy, Ronald, Kim, Edward H, Koo, Neil W, Kowall, Patricia, Kramer, Walter A, Kukull, James J, Lah, Eric B, Larson, Allan I, Levey, Andrew P, Lieberman, Oscar L, Lopez, Kathryn L, Lunetta, Wendy J, Mack, Daniel C, Marson, Eden R, Martin, Frank, Martiniuk, Deborah C, Mash, Eliezer, Masliah, Wayne C, McCormick, Susan M, McCurry, Andrew N, McDavid, Ann C, McKee, Marsel, Mesulam, Bruce L, Miller, Carol A, Miller, Joshua W, Miller, Thomas J, Montine, John C, Morris, Amanda J, Myers, Adam C, Naj, Petra, Nowotny, Joseph E, Parisi, Daniel P, Perl, Elaine, Peskind, Wayne W, Poon, Huntington, Potter, Joseph F, Quinn, Ashok, Raj, Ruchita A, Rajbhandary, Murray, Raskind, Eric M, Reiman, Barry, Reisberg, Christiane, Reitz, John M, Ringman, Erik D, Roberson, Ekaterina, Rogaeva, Roger N, Rosenberg, Mary, Sano, Andrew J, Saykin, Julie A, Schneider, Lon S, Schneider, William, Seeley, Michael L, Shelanski, Michael A, Slifer, Charles D, Smith, Joshua A, Sonnen, Salvatore, Spina, Peter, St George-Hyslop, Robert A, Stern, Rudolph E, Tanzi, John Q, Trojanowski, Juan C, Troncoso, Debby W, Tsuang, Vivianna M, Van Deerlin, Badri Narayan, Vardarajan, Harry V, Vinters, Jean Paul, Vonsattel, Li-San, Wang, Sandra, Weintraub, Kathleen A, Welsh-Bohmer, Jennifer, Williamson, and Randall L, Woltjer

Subjects

Male, Candidate gene, Genotype, Apolipoprotein E4, Gene Dosage, Gene Expression, Single-nucleotide polymorphism, Genome-wide association study, Locus (genetics), Biology, Gene dosage, Polymorphism, Single Nucleotide, PICALM, Alzheimer Disease, Risk Factors, Humans, Genetic Predisposition to Disease, Alleles, Genetic association, Aged, Temporal cortex, Genetics, Brain Chemistry, Temporal Lobe, Linear Models, RNA, Female, Neurology (clinical), Autopsy

Abstract

Objective: Recent genome-wide association studies (GWAS) of late-onset Alzheimer disease (LOAD) identified 9 novel risk loci. Discovery of functional variants within genes at these loci is required to confirm their role in Alzheimer disease (AD). Single nucleotide polymorphisms that influence gene expression (eSNPs) constitute an important class of functional variants. We therefore investigated the influence of the novel LOAD risk loci on human brain gene expression. Methods: We measured gene expression levels in the cerebellum and temporal cortex of autopsied AD subjects and those with other brain pathologies (∼400 total subjects). To determine whether any of the novel LOAD risk variants are eSNPs, we tested their cis -association with expression of 6 nearby LOAD candidate genes detectable in human brain ( ABCA7, BIN1, CLU, MS4A4A, MS4A6A, PICALM ) and an additional 13 genes ±100 kb of these SNPs. To identify additional eSNPs that influence brain gene expression levels of the novel candidate LOAD genes, we identified SNPs ±100 kb of their location and tested for cis -associations. Results: CLU rs11136000 ( p = 7.81 × 10 −4 ) and MS4A4A rs2304933/rs2304935 ( p = 1.48 × 10 −4 –1.86 × 10 −4 ) significantly influence temporal cortex expression levels of these genes. The LOAD-protective CLU and risky MS4A4A locus alleles associate with higher brain levels of these genes. There are other cis -variants that significantly influence brain expression of CLU and ABCA7 ( p = 4.01 × 10 −5 –9.09 × 10 −9 ), some of which also associate with AD risk ( p = 2.64 × 10 −2 –6.25 × 10 −5 ). Conclusions: CLU and MS4A4A eSNPs may at least partly explain the LOAD risk association at these loci. CLU and ABCA7 may harbor additional strong eSNPs. These results have implications in the search for functional variants at the novel LOAD risk loci.

Published

2012

23. Increased miR-708 expression in NSCLC and its association with poor survival in lung adenocarcinoma from never smokers

Author

Fariborz Rakhshan, Jae Yong Park, Debra A. Schultz, Hui Tang, Christopher P. Kolbert, Marie Christine Aubry, Ruth Lupu, Curtis C. Harris, Hyo Sung Jeon, Jin Sung Jang, Cheol Hong Park, Ping Yang, Zhifu Sun, and Jin Jen

Subjects

Cancer Research, Lung Neoplasms, Gene Expression, Kaplan-Meier Estimate, Biology, Adenocarcinoma, Bioinformatics, Article, Cohort Studies, Cell Movement, Carcinoma, Non-Small-Cell Lung, Cell Line, Tumor, Gene expression, microRNA, medicine, Humans, Lung cancer, Wnt Signaling Pathway, Cell Proliferation, Oligonucleotide Array Sequence Analysis, Proportional Hazards Models, Regulation of gene expression, Principal Component Analysis, Oncogene, Gene Expression Profiling, Smoking, Wnt signaling pathway, Membrane Proteins, medicine.disease, Gene expression profiling, Gene Expression Regulation, Neoplastic, MicroRNAs, Oncology, Cancer research, RNA Interference

Abstract

Purpose: miRNA plays an important role in human disease and cancer. We seek to investigate the expression status, clinical relevance, and functional role of miRNA in non–small cell lung cancer. Experimental Design: We conducted miRNA expression profiling in matched lung adenocarcinoma and uninvolved lung using 56 pairs of fresh-frozen (FF) and 47 pairs of formalin-fixed, paraffin-embedded (FFPE) samples from never smokers. The most differentially expressed miRNA genes were evaluated by Cox analysis and log-rank test. Among the best candidate, miR-708 was further examined for differential expression in two independent cohorts. Functional significance of miR-708 expression in lung cancer was examined by identifying its candidate mRNA target and through manipulating its expression levels in cultured cells. Results: Among the 20 miRNAs most differentially expressed between tested tumor and normal samples, high expression level of miR-708 in the tumors was most strongly associated with an increased risk of death after adjustments for all clinically significant factors including age, sex, and tumor stage (FF cohort: HR, 1.90; 95% CI, 1.08–3.35; P = 0.025 and FFPE cohort: HR, 1.93; 95% CI, 1.02–3.63; P = 0.042). The transcript for TMEM88 gene has a miR-708 binding site in its 3′ UTR and was significantly reduced in tumors high of miR-708. Forced miR-708 expression reduced TMEM88 transcript levels and increased the rate of cell proliferation, invasion, and migration in culture. Conclusions: miRNA-708 acts as an oncogene contributing to tumor growth and disease progression by directly downregulating TMEM88, a negative regulator of the Wnt signaling pathway in lung cancer. Clin Cancer Res; 18(13); 3658–67. ©2012 AACR.

Published

2012

24. Effects of joint contracture on the contralateral unoperated limb in a rabbit knee contracture model: a biomechanical and genetic study

Author

Bernard F. Morrey, Kai Nan An, Matthew P. Abdel, Diane E. Grill, Scott P. Steinmann, Joaquin Sanchez-Sotelo, Christopher P. Kolbert, and Mark E. Morrey

Subjects

Flexion contracture, medicine.medical_specialty, Contracture, business.industry, Gene Expression Profiling, Biomechanics, Surgery, Biomechanical Phenomena, body regions, Disease Models, Animal, Lower Extremity, medicine, Rabbit model, Animals, Orthopedics and Sports Medicine, Contralateral limb, Female, Joint Contracture, Rabbits, medicine.symptom, business

Abstract

In most animal models, unoperated contralateral limbs are used as controls. However, in some experimental circumstances, the contralateral limb may represent a skewed control. The main purpose of this study was to determine if the unoperated contralateral limb could be used as a control, or if a different unoperated animal's limb should be used instead. Seventeen rabbits were divided into two groups. Group 1 rabbits (n = 12) underwent surgery on their right limbs to induce a contracture. Group 2 rabbits (n = 5) underwent no surgery. The left non-operated limbs of rabbits in group 1 were biomechanically and genetically compared to the limbs of unoperated rabbits in group 2 with the use of a validated joint measuring device and custom microarray, respectively. After 8 weeks of immobilization, there was a statistically greater flexion contracture in the unoperated contralateral limbs compared to the limbs of animals that received no surgery(8.4 ± 8.9° vs. 0 ± 0°; p-value = 0.03). When animals were remobilized for an additional 16 weeks, the significance between groups was lost (11.9 ± 21.4° vs. 8.9 ± 9.5°; p = 0.38). Similarly, there was a statistically significant increase in nine genes at 8 weeks (p

Published

2011

25. O3‐01‐08: Evaluation of known Alzheimer's genes for SNPs that influence their brain expression (eSNPs)

Author

Neill R. Graff-Radford, Ronald C. Petersen, High Seng Chai, Fanggeng Zou, Thuy Nguyen, Jin Jen, Mariet Allen, Shane Pankratz, Gina Bisceglio, Curtis S. Younkin, Kimberly G. Malphrus, Christopher Rowley, Li Ma, Nilufer Ertekin-Taner, Constantin Georgescu, Asha Nair, Ryan Palusak, Minerva M. Carrasquillo, Sumit Middha, Steven G. Younkin, Dennis W. Dickson, Christopher P. Kolbert, Julia E. Crook, Sooraj Maharjan, and Sarah Lincoln

Subjects

Genetics, Psychiatry and Mental health, Cellular and Molecular Neuroscience, Brain expression, Developmental Neuroscience, Epidemiology, Health Policy, Single-nucleotide polymorphism, Neurology (clinical), Geriatrics and Gerontology, Biology, Gene

Published

2011

26. P1‐229: Genome‐Wide Association Study of Brain Gene Expression Levels (eGWAS)

Author

Kevin Morgan, Harry Campbell, Ozren Polasek, Fanggeng Zou, Shane Pankratz, Caroline Hayward, Clifford R. Jack, Dennis W. Dickson, Sarah Lincoln, Sigrid Botne Sando, Ronald C. Petersen, Ryan Palusak, High Seng Chai, Kimberly G. Malphrus, Neill R. Graff-Radford, Christopher Rowley, Christopher P. Kolbert, Otto Pedraza, Julia E. Crook, Maria Barcikowska, Gina Bisceglio, Thuy Nguyen, Morad Ansari, Jan O. Aasly, Li Ma, Nicholas D. Hastie, Igor Rudan, Sooraj Maharjan, Curtis S. Younkin, Mariet Allen, Zbigniew K. Wszolek, Constantin Georgescu, Nilufer Ertekin-Taner, Asha Nair, Jin Jen, Steven G. Younkin, Alan F. Wright, Minerva M. Carrasquillo, and Sumit Middha

Subjects

Genetics, Psychiatry and Mental health, Cellular and Molecular Neuroscience, Developmental Neuroscience, Epidemiology, Health Policy, Gene expression, Expression quantitative trait loci, Genome-wide association study, Neurology (clinical), Geriatrics and Gerontology, Biology

Published

2011

27. Quantitative miRNA Expression Analysis Using Fluidigm Microfluidics Dynamic Arrays

Author

Fariborz Rakhshan, Jin Sung Jang, Vernadette Simon, Rod M. Feddersen, Debra A. Schultz, Michael A. Zschunke, Wilma L. Lingle, Jin Jen, and Christopher P. Kolbert

Subjects

Tissue Fixation, Microarray, lcsh:QH426-470, lcsh:Biotechnology, Microfluidics, Biology, Polymerase Chain Reaction, Cell Line, Tumor, lcsh:TP248.13-248.65, microRNA, Gene expression, Genetics, Humans, Multiplex, Oligonucleotide Array Sequence Analysis, Cryopreservation, Paraffin Embedding, Methodology Article, Gene Expression Profiling, Molecular biology, Fold change, Gene expression profiling, MicroRNAs, lcsh:Genetics, Real-time polymerase chain reaction, DNA microarray, Biotechnology

Abstract

Background MicroRNAs (miRNAs) represent a growing class of small non-coding RNAs that are important regulators of gene expression in both plants and animals. Studies have shown that miRNAs play a critical role in human cancer and they can influence the level of cell proliferation and apoptosis by modulating gene expression. Currently, methods for the detection and measurement of miRNA expression include small and moderate-throughput technologies, such as standard quantitative PCR and microarray based analysis. However, these methods have several limitations when used in large clinical studies where a high-throughput and highly quantitative technology needed for the efficient characterization of a large number of miRNA transcripts in clinical samples. Furthermore, archival formalin fixed, paraffin embedded (FFPE) samples are increasingly becoming the primary resource for gene expression studies because fresh frozen (FF) samples are often difficult to obtain and requires special storage conditions. In this study, we evaluated the miRNA expression levels in FFPE and FF samples as well as several lung cancer cell lines employing a high throughput qPCR-based microfluidic technology. The results were compared to standard qPCR and hybridization-based microarray platforms using the same samples. Results We demonstrated highly correlated Ct values between multiplex and singleplex RT reactions in standard qPCR assays for miRNA expression using total RNA from A549 (R = 0.98; p < 0.0001) and H1299 (R = 0.95; p < 0.0001) lung cancer cell lines. The Ct values generated by the microfluidic technology (Fluidigm 48.48 dynamic array systems) resulted in a left-shift toward lower Ct values compared to those observed by ABI 7900 HT (mean difference, 3.79), suggesting that the microfluidic technology exhibited a greater sensitivity. In addition, we show that as little as 10 ng total RNA can be used to reliably detect all 48 or 96 tested miRNAs using a 96-multiplexing RT reaction in both FFPE and FF samples. Finally, we compared miRNA expression measurements in both FFPE and FF samples by qPCR using the 96.96 dynamic array and Affymetrix microarrays. Fold change comparisons for comparable genes between the two platforms indicated that the overall correlation was R = 0.60. The maximum fold change detected by the Affymetrix microarray was 3.5 compared to 13 by the 96.96 dynamic array. Conclusion The qPCR-array based microfluidic dynamic array platform can be used in conjunction with multiplexed RT reactions for miRNA gene expression profiling. We showed that this approach is highly reproducible and the results correlate closely with the existing singleplex qPCR platform at a throughput that is 5 to 20 times higher and a sample and reagent usage that was approximately 50-100 times lower than conventional assays. We established optimal conditions for using the Fluidigm microfluidic technology for rapid, cost effective, and customizable arrays for miRNA expression profiling and validation.

Published

2011

28. THE PROTEASOME REGULATES BACTERIAL CpG DNA-INDUCED SIGNALING PATHWAYS IN MURINE MACROPHAGES

Author

Jing Shen, Jian Jun Gao, David C. Morrison, Nilofer Qureshi, Stefanie N. Vogel, Christopher P. Kolbert, Sreekumar Raghavakaimal, Christopher J. Papasian, and Asaf A. Qureshi

Subjects

DNA, Bacterial, Proteasome Endopeptidase Complex, Lactacystin, Biology, Critical Care and Intensive Care Medicine, Article, chemistry.chemical_compound, Mice, Gene expression, medicine, Macrophage, Animals, Gene, Cells, Cultured, Oligonucleotide Array Sequence Analysis, Macrophages, Molecular biology, Proteasome, CpG site, chemistry, Emergency Medicine, Proteasome inhibitor, Female, Signal transduction, medicine.drug, Signal Transduction

Abstract

Our previous work has provided strong evidence that the proteasome is central to the vast majority of genes induced in mouse macrophages in response to lipopolysaccharide (LPS) stimulation. In the studies presented here, we evaluated the role of the macrophage proteasome in response to a second microbial product CpG DNA (unmethylated bacterial DNA). For these studies, we applied Affymetrix microarray analysis of RNA derived from murine macrophages stimulated with CpG DNA in the presence or absence of proteasome inhibitor, lactacystin. The results of these studies revealed that similar to LPS, a vast majority of those macrophage genes regulated by CpG DNA are also under the control of the proteasome at 4 h. In contrast to LPS stimulation, however, many of these genes were induced much later than 4 h, at 18 h, in response to CpG DNA. Lactacystin treatment of macrophages completely blocked the CpG DNA-induced gene expression of TNF-α and other genes involved in production of inflammatory mediators. These data strongly support the conclusion that, similar to LPS, the macrophage proteasome is a key regulator of CpG DNA-induced signaling pathways.

Published

2010

29. Endothelial Nitric Oxide Synthase Gene Variation Associated With Chronic Kidney Disease After Liver Transplant

Author

Cynthia Rys, Christopher P. Kolbert, Rachel A. Pedersen, Charles B. Rosen, Julie M. Cunningham, Kiran Bambha, W. Ray Kim, and Terry M. Therneau

Subjects

Male, medicine.medical_specialty, Genotype, Nitric Oxide Synthase Type III, medicine.medical_treatment, Renal function, Single-nucleotide polymorphism, Kaplan-Meier Estimate, Liver transplantation, Biology, urologic and male genital diseases, Gastroenterology, Polymorphism, Single Nucleotide, Internal medicine, medicine, Humans, Allele, Alleles, Genetic Association Studies, Proportional Hazards Models, Proportional hazards model, Hazard ratio, Homozygote, General Medicine, Middle Aged, medicine.disease, Liver Transplantation, Transplantation, Endocrinology, Kidney Failure, Chronic, Original Article, Female, Kidney disease, Glomerular Filtration Rate

Abstract

OBJECTIVE To identify single nucleotide polymorphisms (SNPs) associated with risk of developing chronic kidney disease (CKD), a prevalent comorbidity, after liver transplant (LT). PATIENTS AND METHODS This study consists of a cohort of adult (≥18 years) primary-LT recipients who had normal renal function before LT and who survived 1 year or more after LT at a high-volume US LT program between January 1, 1990, and December 31, 2000. Patients with adequate renal function (estimated glomerular filtration rate, ≥40 mL/min per 1.73 m 2 during follow-up; n=308) and patients with incident CKD (estimated glomerular filtration rate, 2 after LT; n=92) were identified. To investigate the association of 6 candidate genes with post-LT CKD, we selected SNPs that have been associated with renal function in the literature. Hazard ratios were estimated using Cox regression, adjusted for potential confounding variables. RESULTS The variant allele (298Asp) of the Glu298Asp SNP in the endothelial nitric oxide synthase gene ( NOS3 ) was significantly associated with CKD after LT ( P =.05; adjusted for multiple comparisons). The 5-year incidence of CKD was 70% among patients homozygous for the NOS3 variant allele (298Asp) compared with 42% among those not homozygous for the NOS3 variant allele. Specifically, homozygosity for the NOS3 variant allele conferred a 2.5-fold increased risk of developing CKD after LT ( P =.005, adjusted for confounding variables). CONCLUSION Homozygosity for the variant allele of NOS3 (298Asp) is associated with CKD after LT and may be useful for identifying recipients at higher risk of post-LT CKD.

Published

2010

30. Casp8p41 expression in primary T cells induces a proinflammatory response

Author

Marshall Behrens, Julie A. Taylor, Keith L. Knutson, Andrew D. Badley, Yan W. Asmann, Jane Kahl, Nathan W. Cummins, Stacey A. Rizza, Gary D. Bren, and Christopher P Kolbert

Subjects

Interleukin 2, CD4-Positive T-Lymphocytes, medicine.medical_treatment, Immunology, Blotting, Western, HIV Infections, Biology, Lymphocyte Activation, Virus Replication, Article, Proinflammatory cytokine, Interleukin 21, medicine, Immunology and Allergy, Humans, IL-2 receptor, Interleukin 3, Interleukin-15, Caspase 8, Interleukin-2 Receptor alpha Subunit, NF-kappa B, Molecular biology, Infectious Diseases, Cytokine, Interleukin 15, Interleukin 12, HIV-1, Cytokines, Interleukin-2, medicine.drug

Abstract

Objective HIV infection of CD4 T cells can lead to HIV protease-mediated cleavage of procaspase 8 generating a novel, HIV-specific peptide called Casp8p41. Casp8p41 has at least two biologic functions: induction of cell death via mitochondrial depolarization and release of cytochrome C, as well as activation of nuclear factor kappa B (NFkappaB). We have previously shown that Casp8p41-induced NFkappaB activation enhances HIV LTR transcription and consequently increases HIV replication. Herein, we questioned whether Casp8p41-induced NFkappaB activation impacts the cytokine profile of cells expressing Casp8p41. Design Analysis of cells expressing Casp8p41 and HIV-infected T cells. Methods We assessed whether host genes are transcriptionally activated following Casp8p41 production, using microarray analysis, cytokine quantification, followed by western blot and flow cytometry. Results Microarray analysis identified 259 genes significantly upregulated following expression of Casp8p41. Furthermore, Casp8p41 expression in primary CD4 T cells results in increased production of interleukin (IL)-2, IL-15 and tumor necrosis factor (TNF), as well as IL-1RA; whereas levels of granulocyte macrophage colony-stimulating factor and interferon (IFN)-gamma were reduced in the Casp8p41 expressing cells. Intracellular flow cytometry confirmed the co-association of Casp8p41 with elevated TNF in HIV-infected cells. Conclusion These data indicate that the expression of Casp8p41 in HIV-infected CD4 T cells in addition to promoting apoptosis and enhancing HIV replication also promotes a proinflammatory cytokine milieu, which is characteristic of untreated HIV infection.

Published

2010

31. Identification of Coryneform Bacterial Isolates by Ribosomal DNA Sequence Analysis

Author

Douglas H. Smith, David H. Persing, Christopher P. Kolbert, Marlene K. Hopkins, Alexander von Graevenitz, Stacy O. Montgomery, Haijing Li, Yi-Wei Tang, and Michael Waddington

Subjects

DNA, Bacterial, Microbiology (medical), Genetics, Corynebacterium diphtheriae, Bacilli, Genotype, biology, Microbacterium, Corynebacterium, Bacteriology, Sequence Analysis, DNA, Ribosomal RNA, biology.organism_classification, 16S ribosomal RNA, DNA, Ribosomal, Bacterial Typing Techniques, Microbiology, Evaluation Studies as Topic, Corynebacterium jeikeium, RNA, Ribosomal, 16S, Actinomycetales, Humans, Reagent Kits, Diagnostic, Actinomycetales Infections, Ribosomal DNA

Abstract

Identification of coryneform bacteria to the species level is important in certain circumstances for differentiating contamination and/or colonization from infection, which influences decisions regarding clinical intervention. However, methods currently used in clinical microbiology laboratories for the species identification of coryneform bacteria are often inadequate. We evaluated the MicroSeq 500 16S bacterial sequencing kit (Perkin-Elmer Biosystems, Foster City, Calif.), which is designed to sequence the first 527 bp of the 16S rRNA gene for bacterial identification, by using 52 coryneform gram-positive bacilli from clinical specimens isolated from January through June 1993 at the Mayo Clinic. Compared to conventional and supplemented phenotypic methods, MicroSeq provided concordant results for identification to the genus level for all isolates. At the species level, MicroSeq provided concordant results for 27 of 42 (64.3%) Corynebacterium isolates and 5 of 6 (83.3%) Corynebacterium -related isolates, respectively. Within the Corynebacterium genus, MicroSeq gave identical species-level identifications for the clinically significant Corynebacterium diphtheriae (4 of 4) and Corynebacterium jeikeium (8 of 8), but it identified only 50.0% (15 of 30) of other species ( P < 0.01). Four isolates from the genera Arthrobacter , Brevibacterium , and Microbacterium , which could not be identified to the species level by conventional methods, were assigned a species-level identification by MicroSeq. The total elapsed time for running a MicroSeq identification was 15.5 to 18.5 h. These data demonstrate that the MicroSeq 500 16S bacterial sequencing kit provides a potentially powerful method for the definitive identification of clinical coryneform bacterium isolates.

Published

2000

32. 678 Transcriptomic Changes in Colonic Mucosa in Patients With Campylobacter jejuni Post Infectious Irritable Bowel Syndrome

Author

Cheryl E. Bernard, Christopher P. Kolbert, Paula Carlson, Asha Nair, Bruce W. Eckloff, Michael Camilleri, Madhusudan Grover, Gianrico Farrugia, Purna C. Kashyap, Molly Bisbee, and Fariborz Rakhshan

Subjects

Messenger RNA, Hepatology, biology, Microarray, Gastroenterology, RNA, biology.organism_classification, Campylobacter jejuni, Molecular biology, Microbiology, Transcriptome, Exon, Gene expression, Gene

Abstract

Background: Irritable Bowel Syndrome (IBS) has been associated with changes in the rectosigmoid mucosal expression of immune (TNFSF15, TLRs) and nonimmune (tight junctions, mucus and serotonergic) factors. In a recent microarray based study on Campylobacter jejuni post-infectious IBS (PI-IBS), patients were found to have an increased rectal mucosal expression of CCL11, CCL13, Calpain 8 (pro-inflammatory), GABRE and decreased expression of NR1D1, GPR161. Aim: To determine changes in colonic mucosal RNA expression among patients with C. jejuni PI-IBS in comparison to healthy volunteers using whole transcriptome sequencing. Methods: Sigmoid colonic biopsies were obtained from 5 PI-IBS patients (3 females) and 7 age-matched healthy volunteers (5 females). Biopsies were preserved in RNALater at -80°C. Total RNA was isolated using the RNeasy Plus Mini Kit (Qiagen, Valencia, CA). All samples had RNA Integrity Numbers >7.0. RNA library preparation was performed using the Illumina TruSeq RNA Sample Prep v2 (San Diego, CA) and sequencing was performed as paired-end 51 base reads on an Illumina HiSeq 2000 with 3 samples/ lane using TruSeq SBS Sequencing Kit Version 3. Base calling was performed using Illumina's RTA version 1.12.4.2. Analysis (alignment statistics, in-depth quality control, gene and exon expression, fusion transcripts, and single nucleotide variants) was done using MAP-RSeq v1.2.1.3. Differential expression between samples was done using edgeR algorithm. Results were also compared to our recently published transcriptomic data from rectosigmoid biopsies of IBS-D patients (Am J Physiol 306: G1089-G1098, 2014). Results: Overall, mRNA expressions of 20 genes were changed in patients with C. jejuni PI-IBS as compared to healthy volunteers (P values obtained using false detection rate (FDR) threshold of 5% ranged from 10-5 to 10-9) (Table 1). The genes that stood out as potentially relevant to pathophysiology of PI-IBS included: neurotransmitter-related genes (↑neuropeptide Y receptor type 2, ↑Galanin, ↓nitric oxide synthase 2 (inducible), and ↓indoleamine 2, 3-dioxygenase 1), proteases (↑Secretory leukocyte peptidase inhibitor, ↓Matrix metallopeptidase 3), chemokines (↑chemokine C-C motif ligand 18, ↓chemokine C-X-C motif ligand 10 and 11), carbohydratemetabolism (↑aldolase B, ↑sucrase-isomaltase), ion channels and transporters (↑bestrophin 4, ↑calbindin 2, ↑solute carrier family 3). With the exception of aldolase B expression, there was no overlap with the IBS-D dataset. Conclusion: Transcriptome sequencing of sigmoid colonic mucosa in C. jejuni PI-IBS shows distinct transcriptomic differences from healthy controls and from non-post-infectious IBS-D. These data provide the rationale to explore the role of mucosal factors in the pathophysiology of C. jejuni PI-IBS. Table 1: Gene expression identified by edgeR showing relative expression in C. jejuni PIIBS compared to healthy volunteers

Published

2015

33. Key inflammatory signaling pathways are regulated by the proteasome

Author

Christopher P. Kolbert, Christopher J. Papasian, Jing Shen, Nilofer Qureshi, Asaf A. Qureshi, Julia C Reis, David C. Morrison, Sreekumar Raghavakaimal, and Stefanie N. Vogel

Subjects

Lipopolysaccharides, Proteasome Endopeptidase Complex, Lipopolysaccharide, Cell Survival, medicine.medical_treatment, Lactacystin, Biology, Critical Care and Intensive Care Medicine, Gene Expression Regulation, Enzymologic, Sepsis, chemistry.chemical_compound, Mice, Intensive care, medicine, Animals, Chymotrypsin, Oligonucleotide Array Sequence Analysis, Inflammation, Macrophages, medicine.disease, Shock, Septic, Cell biology, Acetylcysteine, Toll-Like Receptor 4, Cytokine, Proteasome, chemistry, Immunology, Emergency Medicine, Proteasome inhibitor, Signal transduction, medicine.drug, Signal Transduction

Abstract

Lipopolysaccharide (LPS) is a major structural component of all Gram-negative organisms and has been implicated in Gram-negative sepsis and septic shock. In the present study, Affymetrix microarray analysis of RNA derived from murine macrophages treated with LPS in the absence or presence of the proteasome inhibitor lactacystin revealed that the vast majority of genes regulated by LPS is under control of the proteasome. Analysis of the data has revealed that the products of these genes participate in 14 distinct signaling pathways. This represents a novel approach to the identification of signaling pathways that are both toll-like receptor 4- and proteasome-dependent and may lead to the development of new drug targets in Gram-negative sepsis and septic shock.

Published

2006

34. Gene Expression Microarrays

Author

William R. Taylor, Christopher P. Kolbert, Kelly L. Krajnik, and Dennis J. O'Kane

Subjects

Gene expression profiling, Text mining, business.industry, Gene expression microarray, Computational biology, Biology, business

Published

2003

35. Methylmercury induces apoptosis in cultured rat dorsal root ganglion neurons

Author

Anthony J. Windebank, Christopher P. Kolbert, Rod A. Rahimi, and Russell A. Wilke

Subjects

Neurite, Transcription, Genetic, Cell, Apoptosis, Biology, Toxicology, medicine.disease_cause, PC12 Cells, Rats, Sprague-Dawley, Dorsal root ganglion, Pregnancy, Ganglia, Spinal, medicine, Neurites, Animals, Cells, Cultured, Neurons, TUNEL assay, Dose-Response Relationship, Drug, General Neuroscience, Neurotoxicity, Methylmercury Compounds, medicine.disease, In vitro, Cell biology, Rats, medicine.anatomical_structure, Female, Neuroscience, Oxidative stress

Abstract

Methylmercury is known to have devastating effects on the mammalian nervous system. In order to characterize the dose dependence of methylmercury-induced neurotoxicity, we first studied neurite outgrowth from rat dorsal root ganglia explants. In this model, methylmercury inhibited neurite outgrowth with a TD(50) of approximately 0.5 microM. We then used this relationship to optimize dosing for subsequent transcriptional profiling analyses in two independent neuronal model systems: dissociated sensory neurons and PC12 cells. As seen in previous studies, the expression of a number of genes associated with oxidative stress was altered following a 6h challenge with 1 microM methylmercury. When PC12 cells were subjected to a longer exposure (24h), a relative increase was noted in the representation of genes associated with cell cycling and apoptosis. To confirm the presence of apoptosis in cultured neurons, we then applied TUNEL staining and bis-benzimide staining techniques to primary cultures of dissociated sensory neurons. After 24h, 1 microM methylmercury increased both DNA end-labeling (P0.01) and nuclear fragmentation (P0.02). The latter effect appeared to be dose-dependent.

Published

2003

36. Gene expression microarrays

Author

Christopher P, Kolbert, William R, Taylor, Kelly L, Krajnik, and Dennis J, O'Kane

Subjects

DNA, Complementary, Microscopy, Fluorescence, Gene Expression Profiling, Calibration, Humans, Nucleic Acid Hybridization, RNA, DNA, Neoplasm, Cloning, Molecular, Oligonucleotide Probes, Software, Oligonucleotide Array Sequence Analysis

Published

2003

37. Direct identification of bacteria from positive blood cultures by amplification and sequencing of the 16S rRNA gene: evaluation of BACTEC 9240 instrument true-positive and false-positive results

Author

Emily A. Vetter, Christopher P. Kolbert, Qinfang Qian, Stacy O. Montgomery, Franklin R. Cockerill, John G. Hughes, Yi-Wei Tang, W. Scott Harmsen, David H. Persing, and Catherine A. Torgerson

Subjects

Microbiology (medical), DNA, Bacterial, Bacteremia, Biology, Polymerase Chain Reaction, Microbiology, law.invention, Chocolate agar, chemistry.chemical_compound, Leukocyte Count, law, RNA, Ribosomal, 16S, medicine, False positive paradox, Humans, Blood culture, False Positive Reactions, medicine.diagnostic_test, Bacteria, Becton dickinson, Genes, rRNA, Bacteriology, Sequence Analysis, DNA, 16S ribosomal RNA, biology.organism_classification, Molecular biology, Bacterial Typing Techniques, Culture Media, Gram staining, Blood, chemistry, Subculture (biology)

Abstract

In a previous study which evaluated the BACTEC 9240 automated blood culture system (Becton Dickinson Diagnostic Instrument Systems, Sparks, Md.), we noted a 1.3% “instrument false-positive” rate. That is, the BACTEC system signaled that a bottle (BACTEC Plus Aerobic/F bottle or BACTEC Anaerobic Lytic/10 bottle) culture was positive but a Gram stain was negative and there was no growth of bacteria or yeasts on subculture to chocolate agar. Furthermore, from the same sample of blood, cultures for fungi using the Isolator blood culture system (Wampole Laboratories, Cranbury, N.J.) were negative for growth. For the present study, we evaluated 76 instrument false-positive samples for the presence of 16S ribosomal DNA using the MicroSeq 500 kit (PE Biosystems, Foster City, Calif.). These samples also were negative for fungi by the Isolator method. This kit has a PCR module and sequencing module for the amplification and sequencing of the 16S RNA gene and provides a database for sequence alignment and identification of bacteria. To optimize the assay, we evaluated the effect of adding 0.5% bovine serum albumin to the sample from blood culture bottles and found that it decreased the effects of inhibitors on the PCR. Two control groups of blood culture specimens were also evaluated. One group ( n = 45) were “instrument true positives”; the instrument signaled positive, and subsequent Gram stains were positive and subcultures on chocolate agar grew bacteria. The other group ( n = 20) were “instrument true negatives”; the instrument signaled negative, the Gram stain was negative, and subcultures on chocolate agar and from the Isolator tube on fungal media showed no growth. None of the 76 instrument false-positive samples had evidence for 16S rRNA gene sequences. All of the instrument true-positive samples and all of the instrument true-negative specimens were positive and negative, respectively, using the MicroSeq 500 kit. Total peripheral white blood cell counts were statistically significantly higher for patients who had instrument false-positive results than for patients who had instrument true-positive or true-negative results ( P = 0.001). We conclude that instrument false positives signaled by the BACTEC 9240 system are not due to bacteria in the blood culture samples.

Published

2001

38. Direct mecA detection from blood culture bottles by branched-DNA signal amplification

Author

Franklin R. Cockerill, David H. Persing, J. Kolberg, Christopher P. Kolbert, J. Arruda, M. Lewis, Xiaotian Zheng, and P. Varga-Delmore

Subjects

Microbiology (medical), DNA, Bacterial, Micrococcaceae, Staphylococcus, Bacteremia, Biology, Polymerase Chain Reaction, Sensitivity and Specificity, law.invention, Microbiology, Bacterial Proteins, law, Predictive Value of Tests, BDNA test, medicine, Humans, Blood culture, Polymerase chain reaction, medicine.diagnostic_test, SCCmec, virus diseases, Bacteriology, Nucleic acid amplification technique, Staphylococcal Infections, biology.organism_classification, Culture Media, Gram staining, Blood, Subculture (biology), Nucleic Acid Amplification Techniques

Abstract

A branched-DNA (bDNA) signal amplification method was used to detect the mecA gene directly from blood culture broth growing staphylococci. BACTEC blood culture bottles with positive growth indices and containing staphylococcus-like organisms as shown by Gram stain were tested for the presence of the mecA gene. Comparison of test results was done among 225 patients (one blood culture from each patient). Compared with PCR, the sensitivity and specificity of the bDNA method are 100 and 99%, respectively. The bDNA test is carried out in a 96-well format and requires approximately 6 h to perform. Our preliminary results suggest that direct detection of the mecA gene by bDNA signal amplification is (i) sensitive enough to detect mecA directly from blood culture bottles without the requirement for subculture and (ii) as sensitive and specific as the PCR-based method.

Published

1999

39. Clinical significance of TT virus infection in patients with chronic hepatitis C

Author

Haijing Li, Mehmet Arslan, John B. Gross, John J. Poterucha, David H. Persing, Michael Charlton, Christopher P. Kolbert, Nizar N. Zein, and Terry M. Therneau

Subjects

Liver Cirrhosis, Male, medicine.medical_specialty, Cirrhosis, Carcinoma, Hepatocellular, Genotype, Population, Molecular Sequence Data, Hepacivirus, Gastroenterology, Polymerase Chain Reaction, Virus, Liver disease, Internal medicine, medicine, Humans, education, education.field_of_study, Univariate analysis, Hepatology, Base Sequence, business.industry, Liver Neoplasms, DNA Viruses, virus diseases, Hepatitis C, Chronic, Middle Aged, medicine.disease, digestive system diseases, DNA Virus Infections, Hepatocellular carcinoma, Immunology, Female, Viral disease, business

Abstract

OBJECTIVE: The TT virus (TTV) is a novel DNA virus that has recently been identified. The clinical significance of TTV infection in patients with chronic hepatitis C has not been determined. The aim of this study was to determine the prevalence and possible role of TTV in a well characterized population with chronic hepatitis C infection. METHODS: Ninety patients with chronic HCV and known time of HCV acquisition were selected from approximately 250 patients followed at our institution. Characteristics including age, sex, histology, and length of disease were recorded. Direct sequencing of the NS5 region was used for HCV genotyping. TTV DNA detection was based on PCR. RESULTS: TTV infection was present in 24 of 90 (27%) HCV patients. Patients were divided into four groups based on stage of disease; chronic hepatitis (CH, 29 patients), compensated cirrhosis (CC, 17 patients), decompensated cirrhosis (DC, 28 patients), and hepatocellular carcinoma (HCC, 16 patients). TTV was present in 2/29 (7%), 2/17 (12%), 11/28 (39%), and 9/16 (56%) in those with CAH, CC, DC, and HCC respectively. TTV was significantly more prevalent among those with advanced disease (DC and HCC) compared to those with stable disease (CH and CC; p = 0.001). Mean age, sex, and the time from exposure to HCV to development of complications were similar in TTV-positive and -negative patients. TTV infection was more common in patients infected with HCV genotype 1b. Univariate analysis showed that length of HCV infection, HCV genotype 1b, and TTV infection were important in predicting the stage of liver disease in HCV patients. However, after adjusting for length of HCV infection, TTV but not HCV genotype was important in predicting the stage of liver disease. CONCLUSIONS: We conclude that 1) TTV infection is common in patients with chronic HCV; 2) TTV infection is more prevalent among patients with advanced HCV-associated liver disease (DC and HCC) than in those with stable disease (CH and CC); and 3) TTV infection is more common in patients with HCV genotype 1b but is independent from genotype in predicting the stage of HCV-associated liver disease.

Published

1999

40. Comparison of susceptibility testing methods with mecA gene analysis for determining oxacillin (methicillin) resistance in clinical isolates of Staphylococcus aureus and coagulase-negative Staphylococcus spp

Author

Franklin R. Cockerill, Peggy C. Kohner, David H. Persing, Christopher P. Kolbert, and J. R. Uhl

Subjects

Microbiology (medical), Coagulase, Staphylococcus aureus, Meticillin, food.ingredient, Penicillin Resistance, Staphylococcus, Microbial Sensitivity Tests, Biology, Muramoylpentapeptide Carboxypeptidase, Sodium Chloride, medicine.disease_cause, Agar dilution, Microbiology, Minimum inhibitory concentration, food, Bacterial Proteins, medicine, Agar, Humans, Penicillin-Binding Proteins, Antibacterial agent, Oxacillin, SCCmec, Bacteriology, Hexosyltransferases, Genes, Bacterial, Peptidyl Transferases, Carrier Proteins, medicine.drug

Abstract

Ninety-nine clinical staphylococcal isolates (58 coagulase-negative Staphylococcus spp. [CoNS] and 41 Staphylococcus aureus isolates) were evaluated for susceptibility to oxacillin. The following susceptibility testing methods, media, and incubation conditions were studied: agar dilution by using Mueller-Hinton (MH) medium (Difco) supplemented with either 0, 2, or 4% NaCl and incubation at 30 or 35°C in ambient air for 24 or 48 h; disk diffusion by using commercially prepared MH medium (Difco) and MH II agar (BBL) and incubation at 35°C in ambient air for 24 or 48 h; and agar screen (spot or swab inoculation) by using commercially prepared agar (Remel) or MH agar (Difco) prepared in-house, each containing 4% NaCl and 6 μg of oxacillin/ml (0.6-μg/ml oxacillin was also studied with MH agar prepared in-house for the agar swab method and CoNS isolates) and incubation at 35°C in ambient air for 24 or 48 h for swab inoculation and at 30 or 35°C in ambient air for 24 or 48 h for spot inoculation. The results for these methods were compared to the results for mecA gene detection by a PCR method. Given the ability to support growth and the results for susceptibility testing (the breakpoint for susceptible isolates was ≤2 μg/ml), the best methods for CoNS isolates were (i) agar dilution by using MH medium supplemented with 4% NaCl and incubation at 35°C for 48 h (no growth failures were noted, and sensitivity was 97.6%) and (ii) agar screen (swab inoculation) by using MH medium prepared in-house supplemented with 4% NaCl and containing 0.6 μg oxacillin/ml and incubation at 35°C for 48 h (one isolate that did not carry the mecA gene did not grow, and the sensitivity was 100%). All but one (agar dilution without added NaCl and incubation at 30°C for 48 h) of the methods tested revealed all oxacillin-resistant S. aureus isolates, and no growth failures occurred with any method. If the breakpoint for susceptibility was lowered to ≤1 μg/ml for agar dilution methods, more CoNS isolates with oxacillin resistance related to the mecA gene were detected when 0 or 2% NaCl agar supplementation was used. Only one CoNS isolate with mecA gene-associated resistance was not detected by using agar dilution and MH medium supplemented with 4% NaCl with incubation for 48 h. When the breakpoint for susceptibility was decreased 10-fold (from 6.0 to 0.6 μg of oxacillin per ml) for the agar swab screen method, fully 100% of the CoNS isolates that carried the mecA gene were identified.

Published

1999

41. Ribosomal DNA sequencing as a tool for identification of bacterial pathogens

Author

David H. Persing and Christopher P. Kolbert

Subjects

Microbiology (medical), Genetics, DNA, Bacterial, Bacteria, Base Sequence, Sequence Analysis, DNA, Ribosomal RNA, Biology, Microbiology, DNA, Ribosomal, DNA sequencing, Infectious Diseases, Bacterial isolate, RNA, Ribosomal, 16S, Genotype, Humans, Identification (biology), Ribosomal DNA, Sequence (medicine)

Abstract

Conventional methods for the identification and characterization of clinical isolates of bacterial pathogens sometimes fall short when such isolates exhibit unusual phenotypic profiles. Recent advances in DNA sequencing technology have greatly enhanced the ability of the microbiologist to determine the identity of a bacterial isolate. Given the relative objectivity of DNA sequence information and growing availability of sequence information databases, a significant movement is now afoot to use molecular methods for the identification of clinical pathogens.

Published

1999

42. Branched-DNA Assay for Detection of the mecA Gene in Oxacillin-Resistant and Oxacillin-Sensitive Staphylococci

Author

J. Kolberg, J. Arruda, M. Lewis, Christopher P. Kolbert, P. Varga-Delmore, Xiaotian Zheng, and David H. Persing

Subjects

Microbiology (medical), DNA, Bacterial, Penicillin binding proteins, Staphylococcus, Biology, Microbiology, law.invention, Antibiotic resistance, law, BDNA test, polycyclic compounds, Humans, Polymerase chain reaction, Antibacterial agent, DNA Primers, Oxacillin, SCCmec, Nucleic Acid Hybridization, Bacteriology, biochemical phenomena, metabolism, and nutrition, Staphylococcal Infections, Branched DNA assay, Molecular diagnostics, bacterial infections and mycoses, Phenotype, Genes, Bacterial, bacteria, Methicillin Resistance

Abstract

Methicillin resistance in clinical isolates of Staphylococcus is thought to occur as a combined result of the expression of the mecA gene, which codes for the cell wall surrogate enzyme penicillin binding protein (PBP) 2a or 2′ and several factors such as the fem gene series or auxiliary (aux) genes (reviewed in reference 5). In clinical laboratories, antibiotic resistance is usually detected by using methods that require a viable culture of the organism and phenotypic expression of resistance genes. However, studies indicate that there is heterogeneous expression of PBP 2a that is dependent on environmental conditions (1, 10, 16). In addition, some isolates have been shown to exhibit low- or moderate-level methicillin resistance due to overproduction of β-lactamase, modifications in the PBP binding affinities, or the presence of expression factors not related to the mecA gene (2, 9, 12, 20). Variations in laboratory reporting of high-level methicillin resistance, which requires treatment with vancomycin, may be responsible for unnecessary vancomycin usage. The current guidelines from the Centers for Disease Control and Prevention suggest restriction of vancomycin use in order to slow the occurrence of vancomycin resistance in staphylococci (4). Molecular diagnostic assays, which detect genetic targets irrespective of expression level, have proven useful for the identification of isolates containing mecA. In recent years, several genotypic detection methods have been described (3, 7, 11, 14, 17). Most are PCR based, and some are multiplexed with broad-range 16S ribosomal DNA primers to assess the lysis efficiency of each assay. While these assays are highly sensitive and specific, we have found that they are time-consuming and PCR failures may occasionally occur due to lysis inefficiency or inhibitory substances. In the past, assays utilizing branched-DNA (bDNA) technology have been developed to detect antibiotic resistance markers as well as pathogenic agents in clinical samples (6, 19). This assay uses multiple probes that cause an amplification of chemiluminescent signal rather than the amplification of a genetic target that is observed in PCR-based assays. To avoid the complications observed with other tests, we developed a mecA-specific assay that uses bDNA technology to detect the gene in lysates derived from bacterial colonies isolated on solid media and directly from blood cultures. The assay is performed in a 96-well microtiter plate format and takes approximately 6 h to complete, thereby allowing same-day results for cultures containing staphylococci. (Portions of this work were presented at the Conference on Molecular Diagnostics and Therapeutics, Kananaskis, Alberta, Canada, 15–19 August 1997, and the 37th Interscience Conference on Antimicrobial Agents and Chemotherapy, Toronto, Ontario, Canada, 28 September–1 October 1997.)

Published

1998

43. Cosegregation of a novel Bartonella species with Borrelia burgdorferi and Babesia microti in Peromyscus leucopus

Author

Marlene K. Hopkins, David H. Persing, A. Ambyaye, Sam R. Telford, A. S. Abdulkarim, Franklin R. Cockerill, Christopher P. Kolbert, Erick K Hofmeister, James R. Uhl, and J. M. H. Magera

Subjects

Bartonella, DNA, Bacterial, Peromyscus, Minnesota, Spirochaetaceae, Citrate (si)-Synthase, Mice, SCID, Polymerase Chain Reaction, Apicomplexa, Mice, Wisconsin, hemic and lymphatic diseases, Babesiosis, Bartonella Infections, RNA, Ribosomal, 16S, parasitic diseases, medicine, Prevalence, Immunology and Allergy, Animals, Borrelia burgdorferi, Phylogeny, Lyme Disease, Bartonella vinsonii, biology, Ehrlichiosis, Sequence Analysis, DNA, bacterial infections and mycoses, biology.organism_classification, medicine.disease, Virology, Bartonella grahamii, Infectious Diseases, Massachusetts, Population Surveillance, Coinfection, bacteria

Abstract

During surveillance for various tickborne pathogens in the upper Midwest during the summer and early fall of 1995, a Bartonella-like agent was detected in the blood of mice that were concurrently infected with Borrelia burgdorferi or Babesia microti (or both). The organism was isolated in pure culture after inoculation of blood from wild-caught mice into C.B-17 scid/scid mice. Phylogenetic analysis of the 16S rRNA and the citrate synthase genes showed that the novel Bartonella species and a Bartonella isolate from a mouse captured on Martha's Vineyard, Massachusetts, were closely related to each other and secondarily related to Bartonella grahamii and Bartonella vinsonii. Further analysis of Peromyscus leucopus blood and tissue samples demonstrated that the novel Bartonella species was exclusively found in conjunction with B. burgdorferi and B. microti. Patent coinfection with these agents may be relatively frequent in naturally infected mice.

Published

1998

44. Association of MAPT haplotypes with Alzheimer’s disease risk and MAPT brain gene expression levels

Author

Li Ma, Michaela Kachadoorian, Jin Jen, John K Kauwe, Ronald C. Petersen, High Seng Chai, Shubhabrata Mukherjee, Neill R. Graff-Radford, Gina Bisceglio, Christopher P. Kolbert, Julia E. Crook, Fanggeng Zou, Jonathan L. Haines, Minerva M. Carrasquillo, Richard Mayeux, Sarah Lincoln, Thuy Nguyen, V. Shane Pankratz, Siddharth Krishnan, Zachary S. Quicksall, Joseph E. Parisi, Mariet Allen, Dennis W. Dickson, Curtis S. Younkin, Paul K. Crane, Gerard D. Schellenberg, Steven G. Younkin, Nilufer Ertekin-Taner, Margaret A. Pericak-Vance, Kimberly G. Malphrus, and Lindsay A. Farrer

Subjects

medicine.medical_specialty, Neurology, Cognitive Neuroscience, Clinical Neurology, Disease, Progressive supranuclear palsy, 03 medical and health sciences, 0302 clinical medicine, Gene expression, medicine, 030304 developmental biology, Genetic association, Genetics, 0303 health sciences, business.industry, Geriatrics gerontology, FOS: Clinical medicine, Research, Haplotype, Neurosciences, Alzheimer's disease, medicine.disease, Disease risk, Neurology (clinical), business, Neuroscience, 030217 neurology & neurosurgery

Abstract

Introduction: MAPT encodes for tau, the predominant component of neurofibrillary tangles that are neuropathological hallmarks of Alzheimer’s disease (AD). Genetic association of MAPT variants with late-onset AD (LOAD) risk has been inconsistent, although insufficient power and incomplete assessment of MAPT haplotypes may account for this. Methods: We examined the association of MAPT haplotypes with LOAD risk in more than 20,000 subjects (n-cases = 9,814, n-controls = 11,550) from Mayo Clinic (n-cases = 2,052, n-controls = 3,406) and the Alzheimer’s Disease Genetics Consortium (ADGC, n-cases = 7,762, n-controls = 8,144). We also assessed associations with brain MAPT gene expression levels measured in the cerebellum (n = 197) and temporal cortex (n = 202) of LOAD subjects. Six single nucleotide polymorphisms (SNPs) which tag MAPT haplotypes with frequencies greater than 1% were evaluated. Results: H2-haplotype tagging rs8070723-G allele associated with reduced risk of LOAD (odds ratio, OR = 0.90, 95% confidence interval, CI = 0.85-0.95, p = 5.2E-05) with consistent results in the Mayo (OR = 0.81, p = 7.0E-04) and ADGC (OR = 0.89, p = 1.26E-04) cohorts. rs3785883-A allele was also nominally significantly associated with LOAD risk (OR = 1.06, 95% CI = 1.01-1.13, p = 0.034). Haplotype analysis revealed significant global association with LOAD risk in the combined cohort (p = 0.033), with significant association of the H2 haplotype with reduced risk of LOAD as expected (p = 1.53E-04) and suggestive association with additional haplotypes. MAPT SNPs and haplotypes also associated with brain MAPT levels in the cerebellum and temporal cortex of AD subjects with the strongest associations observed for the H2 haplotype and reduced brain MAPT levels (β = -0.16 to -0.20, p = 1.0E-03 to 3.0E-03). Conclusions: These results confirm the previously reported MAPT H2 associations with LOAD risk in two large series, that this haplotype has the strongest effect on brain MAPT expression amongst those tested and identify additional haplotypes with suggestive associations, which require replication in independent series. These biologically congruent results provide compelling evidence to screen the MAPT region for regulatory variants which confer LOAD risk by influencing its brain gene expression.

Published

2014

45. Perpetuation of the agent of human granulocytic ehrlichiosis in a deer tick-rodent cycle

Author

Jacqueline E. Dawson, Cynthia K. Warner, Christopher P. Kolbert, David H. Persing, Paula Katavolos, and Sam R. Telford

Subjects

DNA, Bacterial, Rodent, animal diseases, Molecular Sequence Data, Ehrlichia, Biology, Tick, Mice, Lyme disease, Ticks, biology.animal, Cricetinae, parasitic diseases, medicine, Animals, Humans, Nymph, Mice, Inbred C3H, Multidisciplinary, Base Sequence, Deer, Ehrlichiosis, Deer ticks, biology.organism_classification, medicine.disease, bacterial infections and mycoses, Virology, Arachnid Vectors, Ehrlichiaceae, Mice, Inbred DBA, Female, Research Article

Abstract

A human-derived strain of the agent of human granulocytic ehrlichiosis, a recently described emerging rickettsial disease, has been established by serial blood passage in mouse hosts. Larval deer ticks acquired infection by feeding upon such mice and efficiently transmitted the ehrlichiae after molting to nymphs, thereby demonstrating vector competence. The agent was detected by demonstrating Feulgen-positive inclusions in the salivary glands of the experimentally infected ticks and from field-derived adult deer ticks. White-footed mice from a field site infected laboratory-reared ticks with the agent of human granulocytic ehrlichiosis, suggesting that these rodents serve as reservoirs for ehrlichiae as well as for Lyme disease spirochetes and the piroplasm that causes human babesiosis. About 10% of host-seeking deer ticks were infected with ehrlichiae, and of these, 20% also contained spirochetes. Cotransmission of diverse pathogens by the aggressively human-biting deer tick may have a unique impact on public health in certain endemic sites.

Published

1996

46. Ixodes dammini as a potential vector of human granulocytic ehrlichiosis

Author

P. D. Mitchell, P. Pancholi, J. S. Dumler, David H. Persing, Sam R. Telford, Christopher P. Kolbert, Kurt D. Reed, and J. S. Bakken

Subjects

Male, Ehrlichiosis, Molecular Sequence Data, Ehrlichia, Tick, Polymerase Chain Reaction, Lyme disease, Wisconsin, Borrelia burgdorferi Group, Species Specificity, parasitic diseases, medicine, Immunology and Allergy, Animals, Humans, Borrelia burgdorferi, Dermacentor variabilis, DNA Primers, Lyme Disease, biology, Base Sequence, Ixodes, Middle Aged, bacterial infections and mycoses, biology.organism_classification, medicine.disease, Virology, Insect Vectors, Blotting, Southern, Infectious Diseases, Female, Dermacentor, Granulocytes

Abstract

Little is known about the epidemiology and mode of transmission of the agent of human granulocytic ehrlichiosis (HGE). Analyses of an engorged female Ixodes dammini tick removed from an HGE patient and 101 field-collected I. dammini and Dermacentor variabilis from three Wisconsin counties for Borrelia burgdorferi and Ehrlichia phagocytophila/Ehrlichia equi DNA revealed that the patient tick and 7 of 68 I. dammini ticks from Washburn County collected in 1982 and 1991 were positive for ehrlichial DNA; 10 ticks from the same collections were positive for B. burgdorferi. Two specimens (2.2%) were positive for both organisms. Serologic evidence for exposure to the agent of HGE or its relatives was detected in 3 of 25 Lyme disease patients from the upper Midwest. These data argue that I. dammini is a common vector for transmission of both Lyme disease and HGE.

Published

1995

47. Detection of the Staphylococcal mecA gene by chemiluminescent DNA hybridization

Author

J E Connolly, M J Lee, Christopher P. Kolbert, and David H. Persing

Subjects

Microbiology (medical), DNA, Bacterial, Genotype, Staphylococcus, Microbial Sensitivity Tests, Biology, Staphylococcal infections, Polymerase Chain Reaction, Sensitivity and Specificity, law.invention, Microbiology, Nucleic acid thermodynamics, law, Multiplex polymerase chain reaction, medicine, Humans, Polymerase chain reaction, Bacteriological Techniques, DNA–DNA hybridization, Hybridization probe, SCCmec, Nucleic Acid Hybridization, Staphylococcal Infections, medicine.disease, Molecular biology, Phenotype, Evaluation Studies as Topic, Genes, Bacterial, Luminescent Measurements, Methicillin Resistance, Research Article

Abstract

A new solution-phase DNA hybridization capture assay for the rapid detection of the mecA gene in clinical isolates of Staphylococcus was compared with multiplex PCR and disk diffusion methods. The assay uses a DNA capture probe immobilized on paramagnetic particles and a second DNA probe labeled with an acridinium ester. Bacteria from 24-h cultures are lysed, and the lysates are hybridized with the DNA probes. After magnetic separation to remove unhybridized labeled probe, the mecA gene is detected by the chemiluminescence of the hybridized probe. Four hundred consecutive staphylococcal isolates were assayed, including 147 S. aureus and 253 coagulase-negative Staphylococcus isolates. Among the S. aureus isolates, 14 of 147 were MecA+ by both the hybridization capture assay and PCR; 133 of 147 were MecA negative by both assays (positive and negative predictive values, 100%). Comparison of disk diffusion results with those obtained by genotypic methods indicated that 14 of 147 S. aureus isolates judged to be resistant were positive by both methods; 119 of 147 were Oxs and negative by both genotypic methods (positive and negative predictive values, 50 and 100%, respectively). The remaining 14 S. aureus isolates were MecA- Oxr; among these, 13 were beta-lactamase hyperproducers. For coagulase-negative staphylococci, 130 of 253 were MecA+ by the hybridization capture assay; 129 of 130 of these isolates were positive by PCR (positive and negative predictive values, 99.2 and 100%, respectively). Comparison with the disk diffusion assay showed that 128 of the coagulase-negative MecA+ isolates were Oxr; 111 of 253 were MecA- and Oxs (positive and negative predictive values, 90.8 and 99.1%, respectively). Thirteen coagulase-negative isolates were MecA-Oxr; among these, three were beta-lactamase hyperproducers. Comparison of the hybridization capture assay results with PCR indicates that the DNA hybridization assay is a sensitive and specific test for the detection of the mecA gene in clinical isolates of Staphylococcus.

Published

1995

48. Novel Progressive Supranuclear Palsy (PSP) Risk Loci Variants Associate with Brain Gene Expression Levels (S54.002)

Author

Christopher P. Kolbert, Christopher Rowley, Gina Bisceglio, Steve Younkin, Neil Graff-Radford, Fanggeng Zou, Constantin Georgescu, Asha Nair, Thuy Nguyen, D. Dickson, J. Crook, Sumit Middha, R. C. Petersen, Sooraj Maharjan, Curtis S. Younkin, Nilufer Taner, High Seng Chai, Li Ma, V. Pankratz, Mariet Allen, Jin Jen, Minerva M. Carrasquillo, Ryan Palusak, Kimberly G. Malphrus, Naomi Kouri, and Sarah Lincoln

Subjects

Genetics, Gene expression, medicine, Neurology (clinical), Biology, medicine.disease, Progressive supranuclear palsy

Published

2012

49. Brain Expression Genome-Wide Association Study (eGWAS) Identifies Human Disease-Associated Variants (P05.069)

Author

Nilufer Taner, Christopher P. Kolbert, Thuy Nguyen, Fanggeng Zou, Minerva M. Carrasquillo, Jin Jen, Neil Graff-Radford, Naomi Kouri, Sarah Lincoln, R. C. Petersen, Mariet Allen, Sumit Middha, J. Crook, Li Ma, Curtis S. Younkin, V. Pankratz, Steve Younkin, Ryan Palusak, Kimberly G. Malphrus, High Seng Chai, Gina Bisceglio, Constantin Georgescu, Asha Nair, Christopher Rowley, D. Dickson, and Sooraj Maharjan

Subjects

Brain expression, Human disease, Genome-wide association study, Neurology (clinical), Computational biology, Biology

Published

2012

50. Ribosomal DMA sequencing as a tool for identification of bacterial pathogens

Author

Christopher P Kolbert and David H Persing

Subjects

Microbiology (medical), Infectious Diseases, Microbiology

Published

1999