Frances Louise Lavender
University of Southampton
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Featured researches published by Frances Louise Lavender.
Leukemia | 2003
J J M van Dongen; A W Langerak; Monika Brüggemann; Paul Anthony Stuart Evans; Michael Hummel; Frances Louise Lavender; Eric Delabesse; Frederic Davi; Eduardus Maria Dominicus Schuuring; Ramón García-Sanz; J.H.J.M. van Krieken; J Droese; D. González; Christian Bastard; Helen E. White; Marcel Spaargaren; González M; Antonio Parreira; J. L. Smith; Gareth J. Morgan; Michael Kneba; Elizabeth Macintyre
In a European BIOMED-2 collaborative study, multiplex PCR assays have successfully been developed and standardized for the detection of clonally rearranged immunoglobulin (Ig) and T-cell receptor (TCR) genes and the chromosome aberrations t(11;14) and t(14;18). This has resulted in 107 different primers in only 18 multiplex PCR tubes: three VH–JH, two DH–JH, two Ig kappa (IGK), one Ig lambda (IGL), three TCR beta (TCRB), two TCR gamma (TCRG), one TCR delta (TCRD), three BCL1-Ig heavy chain (IGH), and one BCL2-IGH. The PCR products of Ig/TCR genes can be analyzed for clonality assessment by heteroduplex analysis or GeneScanning. The detection rate of clonal rearrangements using the BIOMED-2 primer sets is unprecedentedly high. This is mainly based on the complementarity of the various BIOMED-2 tubes. In particular, combined application of IGH (VH–JH and DH–JH) and IGK tubes can detect virtually all clonal B-cell proliferations, even in B-cell malignancies with high levels of somatic mutations. The contribution of IGL gene rearrangements seems limited. Combined usage of the TCRB and TCRG tubes detects virtually all clonal T-cell populations, whereas the TCRD tube has added value in case of TCRγδ+ T-cell proliferations. The BIOMED-2 multiplex tubes can now be used for diagnostic clonality studies as well as for the identification of PCR targets suitable for the detection of minimal residual disease.
Leukemia | 2007
J.H.J.M. van Krieken; Anton W. Langerak; Elizabeth Macintyre; Michael Kneba; Elizabeth Hodges; R Garcia Sanz; Gareth J. Morgan; Antonio Parreira; T. J. Molina; José Cabeçadas; P. Gaulard; Bharat Jasani; Josmar García; M. Ott; M L Hannsmann; Françoise Berger; Michael Hummel; Frederic Davi; Monika Brüggemann; Frances Louise Lavender; Eduardus Maria Dominicus Schuuring; Paul Anthony Stuart Evans; Helen E. White; G. Salles; Patricia J. T. A. Groenen; Paula Gameiro; Ch Pott; J J M van Dongen
The diagnosis of malignant lymphoma is a recognized difficult area in histopathology. Therefore, detection of clonality in a suspected lymphoproliferation is a valuable diagnostic criterion. We have developed primer sets for the detection of rearrangements in the B- and T-cell receptor genes as reliable tools for clonality assessment in lymphoproliferations suspected for lymphoma. In this issue of Leukemia, the participants of the BIOMED-2 Concerted Action CT98-3936 report on the validation of the newly developed clonality assays in various disease entities. Clonality was detected in 99% of all B-cell malignancies and in 94% of all T-cell malignancies, whereas the great majority of reactive lesions showed polyclonality. The combined BIOMED-2 results are summarized in a guideline, which can now be implemented in routine lymphoma diagnostics. The use of this standardized approach in patients with a suspect lymphoproliferation will result in improved diagnosis of malignant lymphoma.
Leukemia | 2007
Anton W. Langerak; T. J. Molina; Frances Louise Lavender; D. Pearson; Thomas Flohr; C. Sambade; Ed Schuuring; T Al Saati; J J M van Dongen; J.H.J.M. van Krieken
Lymphoproliferations are generally diagnosed via histomorphology and immunohistochemistry. Although mostly conclusive, occasionally the differential diagnosis between reactive lesions and malignant lymphomas is difficult. In such cases molecular clonality studies of immunoglobulin (Ig)/T-cell receptor (TCR) rearrangements can be useful. Here we address the issue of clonality assessment in 106 histologically defined reactive lesions, using the standardized BIOMED-2 Ig/TCR multiplex polymerase chain reaction (PCR) heteroduplex and GeneScan assays. Samples were reviewed nationally, except 10% random cases and cases with clonal results selected for additional international panel review. In total 75% (79/106) only showed polyclonal Ig/TCR targets (type I), whereas another 15% (16/106) represent probably polyclonal cases, with weak Ig/TCR (oligo)clonality in an otherwise polyclonal background (type II). Interestingly, in 10% (11/106) clear monoclonal Ig/TCR products were observed (types III/IV), which prompted further pathological review. Clonal cases included two missed lymphomas in national review and nine cases that could be explained as diagnostically difficult cases or probable lymphomas upon additional review. Our data show that the BIOMED-2 Ig/TCR multiplex PCR assays are very helpful in confirming the polyclonal character in the vast majority of reactive lesions. However, clonality detection in a minority should lead to detailed pathological review, including close interaction between pathologist and molecular biologist.
Journal of Pediatric Hematology Oncology | 2002
Mamidipudi T. Krishna; Elizabeth Hodges; Frances Louise Lavender; Susan Harris; Andrew R. Gennery; Andrew J. Cant; Brenda Gibson; Rosalie Wilkie; Philip Darbyshire; J. L. Smith
The authors describe two pediatric cases of large granular lymphocytosis presenting early in the second decade of life with neutropenia and sepsis. They are among the youngest described in the literature. This report focuses on the advantages of detailed immunophenotypic and molecular analysis and highlights some of the controversies and uncertainties in the management of these patients, particularly the choice of immunosuppressive therapy. Immunosuppressive therapy in the two children described in this report resulted in improvement of neutropenia and clinical status, but this was not accompanied by the disappearance of the clonal population.
Archive | 2003
Jacobus Johannes Maria Van Dongen; Eduardus Maria Dominicus Schuuring; Jesus San Miquel; Ramon Garzia Sanz; Antonio Parreira; J. L. Smith; Frances Louise Lavender; Gareth John Morgan; Paul Anthony Stuart Evans; Michael Kneba; Michael Hummel; Elizabeth Macintyre; Christian Bastard
Archive | 2003
Dongen Jacobus Johannes Maria Van; Anthonie Willem Langerak; Eduardus Maria Dominicus Schuuring; Miquel Jesus Fernando San; Sanz Ramon Garcia; Antonio Parreira; J. L. Smith; Frances Louise Lavender; Gareth John Morgan; Paul Anthony Stuart Evans; Michael Kneba; Michael Hummel; Elizabeth Macintyre; Christian Bastard; Frederic Davi; Monika Brüggemann
Archive | 2003
Christian Bastard; Paul Anthony Stuart Evans; Sanz Ramon Garzia; Michael Hummel; Michael Kneba; Anthonie Willem Langerak; Frances Louise Lavender; Elizabeth Macintyre; Gareth John Morgan; Antonio Parreira; Miquel Jesus Fernando San; Eduardus Maria Dominicus Schuuring; J. L. Smith; Dongen Jacobus Johannes Maria Van
Archive | 2003
Dongen Jacobus Johannes Maria Van; Anthonie Willem Langerak; Eduardus Maria Dominicus Schuuring; Miquel Jesus Fernando San; Sanz Ramon Garcia; Antonio Parreira; J. L. Smith; Frances Louise Lavender; Gareth John Morgan; Paul Anthony Stuart Evans; Michael Kneba; Michael Hummel; Elizabeth Macintyre; Christian Bastard; Frederic Davi; Monika Brüggemann
Archive | 2003
Dongen Jacobus Johannes Van; Anthonie Willem Langerak; Eduardus Maria Dominicus Schuuring; Miquel Jesus Fernando San; Sanz Ramon Garzia; Antonio Parreira; J. L. Smith; Frances Louise Lavender; Gareth John Morgan; Paul Anthony Stuart Evans; Michael Kneba; Michael Hummel; Elizabeth Macintyre; Christian Bastard; Frederic Davi; Monika Brueggemann
Archive | 2003
Dongen Jacobus Johannes Maria Van; Anthonie Willem Langerak; Eduardus Maria Dominicus Schuuring; Miquel Jesus Fernando San; Sanz Ramon Garcia; Antonio Parreira; J. L. Smith; Frances Louise Lavender; Gareth John Morgan; Paul Anthony Stuart Evans; Michael Kneba; Michael Hummel; Elizabeth Macintyre; Christian Bastard; Frederic Davi; Monika Brüggemann