成人急性白血病诊断时和完全缓解期间降钙素基因的高甲基化。

X Thomas, M H Teillon, A Belhabri, R Rimokh, D Fiere, J P Magaud, E Archimbaud
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引用次数: 14

摘要

降钙素基因的高甲基化已被描述在各种血液恶性肿瘤。为了评估其作为白血病细胞标志物的频率和潜在用途,并检测其潜在的临床相关性,我们采用Southern blot技术和聚合酶链反应(PCR)技术,对180例(> 15岁)新诊断的急性白血病患者,其中包括133例急性髓性白血病(AML)和47例急性淋巴细胞白血病(ALL),在诊断时检测其在白血病母细胞中的存在,使用3组引物(P550, P566, P1400)。放大上游或基因内最常见的超甲基化位点。在AML中,92例(69%)患者在诊断时通过Southern blot检测到高甲基化。36例检测病例中有18例(50%)可通过PCR证实这种高甲基化。高甲基化与该疾病的任何临床或血液学特征均无显著相关性。在ALL中,44例(94%)患者在诊断时通过Southern blot检测到高甲基化。43例检测病例中有33例(77%)可通过PCR证实这种高甲基化。稀释法检测PCR的灵敏度为1 ~ 0.1%。高甲基化与该疾病的任何临床或血液学特征均无显著相关性。7例诊断时PCR阳性,达到细胞学CR的ALL患者可在CR期间进行检测,5例阴性,CR 3 ~ 27个月后未复发,1例CR开始时阳性,自体移植后变为阴性。然而,在最后一次阴性检测3个月后,他在CR 9个月后复发。同时,PCR检测Bcr/Abl也呈阴性。我们得出结论,降钙素基因的高甲基化在成人急性白血病诊断中是常见的,特别是在ALL中。
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Hypermethylation of calcitonin gene in adult acute leukemia at diagnosis and during complete remission.

Hypermethylation of the calcitonin gene has been described in various hematologic malignancies. In order to assess its frequency and potential usefulness as a marker for leukemic cells and to detect potential clinical correlations, 180 adult patients (aged > 15 years) with newly diagnosed acute leukemia including 133 cases of acute myeloid leukemia (AML) and 47 cases of acute lymphoblastic leukemia (ALL) were tested for its presence in leukemic blasts at diagnosis by Southern blot technique and polymerase chain reaction (PCR) using 3 sets of primers (P550, P566, P1400), amplifying the most frequent sites of hypermethylation upstream or within the gene. In AML, 92 patients (69%) had hypermethylation detected by Southern blot at diagnosis. This hypermethylation could be confirmed by PCR in 18 of 36 tested cases (50%). Hypermethylation was not significantly associated to any clinical or hematological characteristic of the disease. In ALL, 44 patients (94%) had hypermethylation detected by Southern blot at diagnosis. This hypermethylation could be confirmed by PCR in 33 of the 43 tested cases (77%). Sensitivity of PCR assessed by dilution was 1 to 0.1%. Hypermethylation was not either significantly related to any clinical or hematologic characteristics of the disease. Seven ALL cases which were positive by PCR at diagnosis and achieved cytological CR could be tested during CR. Five cases were negative and did not relapse after 3 to 27 months in CR. One case was positive at the beginning of CR and became negative after autologous transplant. However, he relapsed after 9 months in CR, 3 months after the last negative test. PCR for Bcr/Abl was also negative at this time. We conclude that hypermethylation of the calcitonine gene is frequent at diagnosis in adult acute leukemia, particularly in ALL.

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