5 results on '"María Dolores Fellner"'
Search Results
2. Duplex realtime PCR method for Epstein–Barr virus and human DNA quantification: its application for post-transplant lymphoproliferative disorders detection
- Author
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Karina Durand, Marcelo Rodriguez, María Alejandra Picconi, Virginia Alonio, Lucía Irazu, and María Dolores Fellner
- Subjects
Male ,Epstein-Barr Virus Infections ,Herpesvirus 4, Human ,lcsh:QR1-502 ,Ciencias de la Salud ,Transplant ,medicine.disease_cause ,lcsh:Microbiology ,chemistry.chemical_compound ,hemic and lymphatic diseases ,Viral load ,Child ,Medicine(all) ,Middle Aged ,viral load ,surgical procedures, operative ,Infectious Diseases ,Real-time polymerase chain reaction ,Child, Preschool ,purl.org/becyt/ford/3 [https] ,Female ,Adult ,Microbiology (medical) ,CIENCIAS MÉDICAS Y DE LA SALUD ,Adolescent ,Lymphoproliferative disorders ,Biology ,Real-Time Polymerase Chain Reaction ,Sensitivity and Specificity ,Peripheral blood mononuclear cell ,Virus ,lcsh:Infectious and parasitic diseases ,purl.org/becyt/ford/3.3 [https] ,Young Adult ,EBV ,Quantification ,medicine ,Humans ,lcsh:RC109-216 ,Gene ,Salud Ocupacional ,Infant ,medicine.disease ,Kidney Transplantation ,Virology ,Epstein–Barr virus ,Lymphoproliferative Disorders ,Liver Transplantation ,Real time PCR ,PTLD ,chemistry ,DNA, Viral ,Immunology ,Heart Transplantation ,real-time PCR ,DNA - Abstract
INTRODUCTION: The quantification of circulating Epstein-Barr virus (EBV) DNA is used to monitor transplant patients as an early marker of Post-Transplant Lymphoproliferative Disorders (PTLD). So far no standardized methodology exists for such determination. OBJECTIVE: Our purpose was to develop and validate a real-time PCR assay to quantify EBV DNA in clinical samples from transplant recipients. METHODS: A duplex real-time PCR method was developed to amplify DNA from EBV and from a human gene. The EBV load was determined in peripheral blood mononuclear cells (PBMC), plasma and oropharyngeal tissue from 64 non-transplanted patients with lymphoid-hypertrophy (Non-Tx), 47 transplant recipients without PTLD (Tx), 54 recipients with PTLD (Tx-PTLD), and 66 blood donors (BD). WinPEPI, version 11.14 software was used for statistical analysis. RESULTS: Analytical validation: the intra and inter-assays variation coefficients were less than 4.5% (EBV-reaction) and 3% (glyceraldehyde 3-phosphate dehydrogenase - GAPDH reaction). Linear ranges comprised 10(7)-10 EBV genome equivalents (gEq) (EBV-reaction) and 500,000-32 human gEq (GAPDH-reaction). The detection limit was 2.9 EBV gEq (EBV-reaction). Both reactions showed specificity. Application to clinical samples: higher levels of EBV were found in oropharyngeal tissue from transplanted groups with and without PTLD, compared to Non-Tx (p
- Published
- 2014
3. Epstein Barr virus genotypes and LMP-1 variants in HIV-infected patients
- Author
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María Dolores Fellner, Gustavo Sevlever, Virginia Alonio, María Alejandra Picconi, Antonio Colobraro, Karina Durand, Jorge Benetucci, Claudio Yampolsky, Angélica R. Teyssié, Rita Mariel Correa, and Liliana Redini
- Subjects
Adult ,Male ,Epstein-Barr Virus Infections ,Herpesvirus 4, Human ,Adolescent ,Biopsy ,Argentina ,HIV Infections ,medicine.disease_cause ,Polymerase Chain Reaction ,Herpesviridae ,Virus ,law.invention ,Central Nervous System Neoplasms ,Viral Matrix Proteins ,Species Specificity ,law ,hemic and lymphatic diseases ,Virology ,Genotype ,medicine ,Gammaherpesvirinae ,Humans ,Polymerase chain reaction ,Lymphoma, AIDS-Related ,Sequence Deletion ,Acquired Immunodeficiency Syndrome ,biology ,Base Sequence ,Primary central nervous system lymphoma ,Brain ,Genetic Variation ,HIV ,Middle Aged ,biology.organism_classification ,medicine.disease ,Epstein–Barr virus ,Lymphoma ,Blotting, Southern ,Infectious Diseases ,Immunology ,Leukocytes, Mononuclear - Abstract
Two Epstein Barr virus (EBV) genotypes: EBV-1 and EBV-2 have been described. A 30-bp deletion in latent membrane protein-1 gene (del-LMP-1) has been identified in various pathologies. The aim of this study was to determine EBV genotypes and 30-bp deletion frequency in HIV-infected patients from Argentina. The study was performed on 258 individuals: Cases: 144 HIV-infected patients that included: (a) 7 AIDS patients with primary central nervous system lymphoma (PCNSL), (b) 62 AIDS patients, and (c) 75 asymptomatic HIV-infected patients. Controls: 114 HIV-negative individuals. EBV genotypes and variants in LMP-1 gene were detected by polymerase chain reaction (PCR)-Southern blot on DNA extracted from peripheral blood mononuclear cells and brain biopsies. In PCNSL, the presence of EBV was confirmed by EBER RNA in situ hybridization, and DNA sequencing of 3′ end LMP-l gene of PCR products was performed. In HIV-infected patients, EBV-1 was detected in 48.6%, EBV-2 in 18.8%, and co-infection with both genotypes in 32.6%. In control group, EBV-1 was present in 74.3%, EBV-2 in 12.4%, and co-infection in 13.3%. Del-LMP-1 was found in 44.4% of HIV-infected patients samples (20.7% alone and 23.7% co-infection with non-deleted form) while it was found in 25.3% (6.3% alone and 19% with co-infection) in HIV-negative individuals. In HIV-infected patients EBV-2, co-infection and 30-bp deletion are more prevalent than in control group. In all, PCNSL brain biopsies samples, del-LMP-1 always was detected with EBV-2, but more cases would have to be included to draw definitive conclusions. J. Med. Virol. 79:401–407, 2007. © 2007 Wiley-Liss, Inc.
- Published
- 2007
4. Epstein-barr virus (EBV) in healthy carriers: Distribution of genotypes and 30 bp deletion in latent membrane protein-1 (LMP-1) oncogene
- Author
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Rita Mariel, Correa, María Dolores, Fellner, Lidia Virginia, Alonio, Karina, Durand, Angélica R, Teyssié, and María Alejandra, Picconi
- Subjects
Adult ,Male ,Epstein-Barr Virus Infections ,Herpesvirus 4, Human ,Adolescent ,Genotype ,Argentina ,Genetic Variation ,Blood Donors ,Middle Aged ,Polymerase Chain Reaction ,Viral Matrix Proteins ,Carrier State ,Leukocytes, Mononuclear ,Prevalence ,Humans ,Female ,Aged ,Sequence Deletion - Abstract
There are two types of Epstein Barr virus (EBV): EBV-1 and EBV-2, distinguished by genomic polymorphism in the genes encoding the nuclear antigens (EBNA-2, -3A, -3B, -3C). Latent membrane protein 1 (LMP-1) is an EBV protein with known oncogenic properties. Different variants had been described; among them, a 30 base pair (bp) deletion (del-LMP-1) had been reported in benign and malignant pathologies, but there is little information about its frequency in healthy populations. The aim of this study was to determine the distribution of the EBV genotypes and the 30 bp deletion frequency, in EBV healthy carriers from Argentina. Analysis of EBNA-3C and LMP-1 genes were done by polymerase chain reaction (PCR) followed by Southern blot hybridization on DNA of peripheral blood mononuclear cells (PBMCs) from blood bank donors. EBV-1 was present in 75.9% of samples, EBV-2 in 14.6%, and co-infections with both types in 6.5%. The deleted LMP-1 variant was found in 7.4% of analyzed samples, corresponding 3.2% to deleted variant alone and 4.2% to co-infections with non-deleted form. The non-deleted variant was found in 64.6% whereas in the remaining 28%, no PCR product was detected. These results showed that EBV-1 was the more prevalent type in healthy carriers of Argentina, similar to reports from others countries. A predominance of the non-deleted LMP-1 variant was observed. The presence of co-infections with both types and variants demonstrated that healthy individuals may also harbor multiple EBV infections.
- Published
- 2004
5. A semiquantitative PCR method (SQ-PCR) to measure Epstein-Barr virus (EBV) load: its application in transplant patients
- Author
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Mariel Correa, Lidia Virginia Alonio, María Alejandra Picconi, Angélica R. Teyssié, David Bes, Karina Durand, and María Dolores Fellner
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Adult ,Herpesvirus 4, Human ,Adolescent ,Lymphoproliferative disorders ,Biology ,medicine.disease_cause ,Asymptomatic ,Peripheral blood mononuclear cell ,Polymerase Chain Reaction ,Sensitivity and Specificity ,Predictive Value of Tests ,Virology ,medicine ,Humans ,Child ,Viral Load ,medicine.disease ,Epstein–Barr virus ,Kidney Transplantation ,Lymphoproliferative Disorders ,Liver Transplantation ,Infectious Diseases ,Predictive value of tests ,Child, Preschool ,Immunology ,DNA, Viral ,Leukocytes, Mononuclear ,Transplant patient ,medicine.symptom ,Nested polymerase chain reaction ,Viral load - Abstract
High Epstein-Barr virus load has been related to an increased risk of Posttransplant Lymphoproliferative Disorders (PTLD) in transplant recipients.Development of a method to quantitate EBV DNA levels in peripheral blood mononuclear cells (PBMC) and evaluate its usefulness in transplant patients.We designed a semiquantitative nested PCR based on a limiting dilution analysis to detect high viral loads in PBMC. This method was applied to 25 healthy carriers, and 85 solid organ transplant recipients as follows: (A) 53 asymptomatic patients; (B) 24 symptomatic patients; (C) eight patients with PTLD.In healthy carriers the reciprocal of the limiting dilution (RLD) ranged between non-detected (ND) and 1, the median RLD was ND, which is equivalent to a viral load of1 copy per 10(5) PBMC. In the transplant population the medians RLD (range) were: (A) asymptomatic group: ND (ND-64), median equivalent to a viral load of1 copy per 10(5) PBMC; (B) symptomatic group: 4 (ND-256), median equivalent to a range of viral load of 4-64 copies per 10(5) PBMC. (C) PTLD group: 256 (16-16384), median equivalent to a range of viral load of 256-4096 copies per 10(5) PBMC. Statistically significant differences were found between all groups: A+B vs. C (P0.0001); A vs. B (P0.0001); A vs. C (P0.0001), B vs. C (P0.0001). We also observed a good correlation between viral loads and clinical findings in four follow-up patients. Considering the RLD=256 as a cutoff point to detect transplant patients with PTLD, resulted in sensitivity 75%, specificity 96.7%, positive predictive value 60%, negative predictive value 98.3%.This SQ-PCR method enables us to differentiate between transplant patients with and without PTLD; therefore, it could be applied as a marker for early detection of this pathology.
- Published
- 2003
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