Literature DB >> 12411590

Quantification of bcl-2/JH fusion sequences and a control gene by multiplex real-time PCR coupled with automated amplicon sizing by capillary electrophoresis.

Beatriz Sanchez-Vega1, Francisco Vega, L Jeffrey Medeiros, Ming S Lee, Rajyalakshmi Luthra.   

Abstract

Follicular lymphoma is characterized by the presence of the t(14;18)(q32;q21) chromosomal translocation which juxtaposes the bcl-2 gene at 18q21 with the immunoglobulin heavy chain locus at 14q32. Quantification of t(14;18) carrying cells in FL patients can be achieved by real-time PCR, a highly sensitive technique for evaluating treatment efficacy and minimal residual disease. Despite the many advantages of real-time technology for this purpose, one disadvantage is that current real-time t(14;18) PCR assays amplify a control gene as a normalizer in a separate reaction. Since each PCR reaction has its own kinetics, separate PCR assays for target and control sequences can potentially result in inaccurate quantification of t(14;18)-positive cells. In addition, the real-time t(14;18) PCR assays do not determine the size of the amplified fusion sequence, which is helpful for excluding contamination and is commonly used to demonstrate clonal identity between pre- and post-treatment specimens from a patient. To address these limitations, we designed a multiplex real-time PCR protocol that allows amplification of control and target genes in the same reaction and precise size determination of bcl-2/JH fusion sequences by capillary electrophoresis. This multiplex PCR assay is equally sensitive to previous assays, allows more accurate quantification of bcl-2/JH fusion sequences, and is more convenient.

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Year:  2002        PMID: 12411590      PMCID: PMC1907359          DOI: 10.1016/S1525-1578(10)60707-6

Source DB:  PubMed          Journal:  J Mol Diagn        ISSN: 1525-1578            Impact factor:   5.568


  27 in total

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Journal:  Ann Oncol       Date:  1999-11       Impact factor: 32.976

2.  5'-->3' exonuclease-based real-time PCR assays for detecting the t(14;18)(q32;21): a survey of 162 malignant lymphomas and reactive specimens.

Authors:  O C Estalilla; L J Medeiros; J T Manning; R Luthra
Journal:  Mod Pathol       Date:  2000-06       Impact factor: 7.842

3.  A sequence of immuno-chemotherapy with Rituximab, mobilization of in vivo purged stem cells, high-dose chemotherapy and autotransplant is an effective and non-toxic treatment for advanced follicular and mantle cell lymphoma.

Authors:  M Lazzarino; L Arcaini; P Bernasconi; E P Alessandrino; L Gargantini; R Cairoli; E Orlandi; C Astori; E Brusamolino; G Pagnucco; A A Colombo; S Calatroni; I Iacona; M B Regazzi; E Morra
Journal:  Br J Haematol       Date:  2002-01       Impact factor: 6.998

4.  Monitoring of minimal residual disease after CHOP and rituximab in previously untreated patients with follicular lymphoma.

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5.  Quantitative detection of t(14;18)-positive cells by real-time quantitative PCR using fluorogenic probes.

Authors:  L Dölken; F Schüler; G Dölken
Journal:  Biotechniques       Date:  1998-12       Impact factor: 1.993

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7.  Rituximab (anti-CD20 monoclonal antibody) as single first-line therapy for patients with follicular lymphoma with a low tumor burden: clinical and molecular evaluation.

Authors:  P Colombat; G Salles; N Brousse; P Eftekhari; P Soubeyran; V Delwail; E Deconinck; C Haïoun; C Foussard; C Sebban; A Stamatoullas; N Milpied; F Boué; B Taillan; P Lederlin; A Najman; C Thièblemont; F Montestruc; A Mathieu-Boué; A Benzohra; P Solal-Céligny
Journal:  Blood       Date:  2001-01-01       Impact factor: 22.113

8.  Real-Time t(14;18)(q32;q21) PCR assay combined with high-resolution capillary electrophoresis: a novel and rapid approach that allows accurate quantitation and size determination of bcl-2/JH fusion sequences.

Authors:  Beatriz Sanchez-Vega; Francisco Vega; Seema Hai; L Jeffrey Medeiros; Rajyalakshmi Luthra
Journal:  Mod Pathol       Date:  2002-04       Impact factor: 7.842

9.  A novel method to compensate for different amplification efficiencies between patient DNA samples in quantitative real-time PCR.

Authors:  J Meijerink; C Mandigers; L van de Locht; E Tönnissen; F Goodsaid; J Raemaekers
Journal:  J Mol Diagn       Date:  2001-05       Impact factor: 5.568

10.  A validated real-time quantitative PCR approach shows a correlation between tumor burden and successful ex vivo purging in follicular lymphoma patients.

Authors:  M Ladetto; S Sametti; J W Donovan; D Ferrero; M Astolfi; M Mitterer; I Ricca; D Drandi; P Corradini; P Coser; A Pileri; J G Gribben; C Tarella
Journal:  Exp Hematol       Date:  2001-02       Impact factor: 3.084

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  5 in total

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Authors:  Rajyalakshmi Luthra; L Jeffrey Medeiros
Journal:  J Mol Diagn       Date:  2004-08       Impact factor: 5.568

2.  Association of clinical status of follicular lymphoma patients after autologous stem cell transplant and quantitative assessment of lymphoma in blood and bone marrow as measured by SYBR Green I polymerase chain reaction.

Authors:  Nancy Pennell; Anthony Woods; Marciano Reis; Rena Buckstein; David Spaner; Kevin Imrie; Karen Hewitt; Angela Boudreau; Arun Seth; Neil L Berinstein
Journal:  J Mol Diagn       Date:  2006-02       Impact factor: 5.568

3.  Demonstration of array-based analysis for highly multiplexed PCR assays application to detection of IGH@-BCL2 translocations in FFPE follicular lymphoma specimens.

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Journal:  J Mol Diagn       Date:  2011-05       Impact factor: 5.568

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Journal:  Blood       Date:  2008-04-14       Impact factor: 22.113

5.  Simultaneous detection and characterization of toxigenic Clostridium difficile directly from clinical stool specimens.

Authors:  Hanjiang Lai; Chen Huang; Jian Cai; Julian Ye; Jun She; Yi Zheng; Liqian Wang; Yelin Wei; Weijia Fang; Xianjun Wang; Yi-Wei Tang; Yun Luo; Dazhi Jin
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