Reliable quantification of hematopoietic chimerism after allogeneic transplantation for acute leukemia using amplification by real-time PCR of null alleles and insertion/deletion polymorphisms

被引:0
|
作者
A Jiménez-Velasco
M Barrios
J Román-Gómez
G Navarro
I Buño
J A Castillejo
A I Rodríguez
G García-Gemar
A Torres
A I Heiniger
机构
[1] Carlos Haya Hospital,Hematology Department
[2] Reina Sofía Hospital,Hematology Department
[3] Gregorio Marañón Hospital,Bone Marrow Transplantation Unit
来源
Leukemia | 2005年 / 19卷
关键词
chimerism; real-time PCR; acute leukaemia; allogeneic SCT; insertion/deletion polymorphisms;
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摘要
Increasing mixed chimerism (MC) after allogeneic stem cell transplantation (SCT) has been associated with a high risk of relapse in acute leukemia. We evaluated a new method for chimerism detection, based on the quantitative real-time PCR (qrt-PCR) amplification of null alleles or insertion/deletion polymorphisms (indels). All qrt-PCR assays with null alleles and indels attained a sensitivity of at least 10−4, as well as good intra- and interassay concordance, and a high accuracy in experiments with cell mixtures. Informativeness was found in 80.3% of the 61 donor/recipient pairs tested. Nonrelapsed patients showed a progressive decrease in peripheral blood chimerism to values below 0.01% (complete chimerism (CC)). Bone marrow chimerism failed to reach CC more than 4 years after SCT. Increasing MC was observed prior to relapse in 88.2% of patients. Compared with conventional PCR amplification of variable number of tandem repeats, qrt-PCR predicted a significantly higher number of relapses (88.2 vs 44.4%) with a median anticipation period of 58 days. In conclusion, chimerism determination by qrt-PCR amplification of null alleles and indels constitutes a useful tool for the follow-up of patients with acute leukemia after SCT, showing better results than those obtained with conventional PCR.
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页码:336 / 343
页数:7
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