Primers and protocols for standardized detection of minimal residual disease in acute lymphoblastic leukemia using immunoglobulin and T cell receptor gene rearrangements and TAL1 deletions as PCR targets -: Report of the BIOMED-1 CONCERTED ACTION:: Investigation of minimal residual disease in acute leukemia

被引:289
作者
Pongers-Willemse, MJ
Seriu, T
Stolz, F
d'Aniello, E
Gameiro, P
Pisa, P
Gonzalez, M
Bartram, CR
Panzer-Grümayer, ER
Biondi, A
San Miguel, JF
van Dongen, JJM
机构
[1] Erasmus Univ, Univ Rotterdam Hosp, Dept Immunol, NL-3000 DR Rotterdam, Netherlands
[2] Univ Heidelberg, Inst Human Genet, Heidelberg, Germany
[3] St Anna Kinderspital, Childrens Canc Res Inst, Vienna, Austria
[4] Univ Milan, Osped San Gerardo, Dept Pediat, Monza, Italy
[5] Inst Portugues Oncol, Dept Hematol, Lisbon, Portugal
[6] Karolinska Hosp, Dept Hematol, S-10401 Stockholm, Sweden
[7] Hosp Clin Univ, Dept Hematol, Salamanca, Spain
关键词
BIOMED-1; MRD; PCR primers; immunoglobulin genes; T cell receptor genes; junctional region; TAL1; deletion;
D O I
10.1038/sj.leu.2401245
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
It is now widely accepted that the detection of minimal residual disease (MRD) has prognostic value in acute leukemia. However clinical MRD studies need standardized techniques. Therefore, several European laboratories have aligned their goals and performed comparative studies to achieve optimization and standardization of MRD techniques. This was achieved via the BIOMED-1 Concerted Action "Investigation of minimal residual disease in acute leukemia: International standardization and clinical evaluation." This report describes the development of PCR primers and protocols for the detection of MRD in acute lymphoblastic leukemia (ALL) using clone-specific junctional regions of immunoglobulin and T cell receptor gene rearrangements and TALI deletions as PCR targets. A total of 54 primers was developed (1) to amplify rearrangements of the TCRD, TCRG, and IGK (Kde) genes as well as TAL1 deletions; (2) to sequence the junctional regions and breakpoint fusion regions; and (3) to perform MRD detection in bone marrow or peripheral blood samples during follow-up of ALL patients. Protocols were established to identify PCR targets at diagnosis by performing 25 PCR reactions per patient using appropriate positive and negative controls. Standardized protocols were developed for MRD monitoring via single amplification of the PCR target followed by dot blot hybridization with the corresponding patient-specific junctional region probe. In addition, alternative approaches were designed for cases where the target sensitivity of at least 10(-4) was not obtained. The standardization described here of MRD-PCR techniques is essential for the process of translating WIRD research into clinical practice.
引用
收藏
页码:110 / 118
页数:9
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