Mrózek K, Prior T W, Edwards C, Marcucci G, Carroll A J, Snyder P J, Koduru P R, Theil K S, Pettenati M J, Archer K J, Caligiuri M A, Vardiman J W, Kolitz J E, Larson R A, Bloomfield C D
Division of Hematology and Oncology, Comprehensive Cancer Center, Ohio State University, Columbus, OH 43210-1228, USA.
J Clin Oncol. 2001 May 1;19(9):2482-92. doi: 10.1200/JCO.2001.19.9.2482.
To prospectively compare cytogenetics and reverse transcriptase-polymerase chain reaction (RT-PCR) for detection of t(8;21)(q22;q22) and inv(16)(p13q22)/t(16;16)(p13;q22), aberrations characteristic of core-binding factor (CBF) acute myeloid leukemia (AML), in 284 adults newly diagnosed with primary AML.
Cytogenetic analyses were performed at local laboratories, with results reviewed centrally. RT-PCR for AML1/ETO and CBFbeta/MYH11 was performed centrally.
CBF AML was ultimately identified in 48 patients: 21 had t(8;21) or its variant and AML1/ETO, and 27 had inv(16)/t(16;16), CBFbeta/MYH11, or both. Initial cytogenetic and RT-PCR analyses correctly classified 95.7% and 96.1% of patients, respectively (P =.83). Initial cytogenetic results were considered to be false-negative in three AML1/ETO-positive patients with unique variants of t(8;21), and in three CBFbeta/MYH11-positive patients with, respectively, an isolated +22; del(16)(q22),+22; and a normal karyotype. The latter three patients were later confirmed to have inv(16)/t(16;16) cytogenetically. Only one of 124 patients reported initially as cytogenetically normal was ultimately RT-PCR-positive. There was no false-positive cytogenetic result. Initial RT-PCR was falsely negative in two patients with inv(16) and falsely positive for AML1/ETO in two and for CBFbeta/MYH11 in another two patients. Two patients with del(16)(q22) were found to be CBFbeta/MYH11-negative. M4Eo marrow morphology was a good predictor of the presence of inv(16)/t(16;16).
Patients with t(8;21) or inv(16) can be successfully identified in prospective multi-institutional clinical trials. Both cytogenetics and RT-PCR detect most such patients, although each method has limitations. RT-PCR is required when the cytogenetic study fails; it is also required to determine whether patients with suspected variants of t(8;21), del(16)(q22), or +22 represent CBF AML. RT-PCR should not replace cytogenetics and should not be used as the only diagnostic test for detection of CBF AML because of the possibility of obtaining false-positive or false-negative results.
前瞻性比较细胞遗传学和逆转录聚合酶链反应(RT-PCR)在284例新诊断的原发性急性髓系白血病(AML)成年患者中检测t(8;21)(q22;q22)和inv(16)(p13q22)/t(16;16)(p13;q22)的情况,这两种异常是核心结合因子(CBF)急性髓系白血病的特征性表现。
细胞遗传学分析在当地实验室进行,结果集中审核。AML1/ETO和CBFβ/MYH11的RT-PCR检测在中心实验室进行。
最终在48例患者中鉴定出CBF AML:21例有t(8;21)或其变异型以及AML1/ETO,27例有inv(16)/t(16;16)、CBFβ/MYH11或两者皆有。初始细胞遗传学和RT-PCR分析分别正确分类了95.7%和96.1%的患者(P = 0.83)。在3例具有独特t(8;21)变异型的AML1/ETO阳性患者以及3例分别具有孤立的+22;del(16)(q22),+22;和正常核型的CBFβ/MYH11阳性患者中,初始细胞遗传学结果被认为是假阴性。后3例患者后来经细胞遗传学证实有inv(16)/t(16;16)。最初报告细胞遗传学正常的124例患者中只有1例最终RT-PCR呈阳性。没有假阳性的细胞遗传学结果。2例inv(16)患者的初始RT-PCR为假阴性,另有2例AML1/ETO和2例CBFβ/MYH11的RT-PCR为假阳性。2例del(16)(q22)患者被发现CBFβ/MYH11为阴性。M4Eo骨髓形态是inv(16)/t(16;16)存在的良好预测指标。
在多机构前瞻性临床试验中可以成功鉴定出有t(8;21)或inv(16)的患者。细胞遗传学和RT-PCR都能检测出大多数此类患者,尽管每种方法都有局限性。当细胞遗传学研究失败时需要进行RT-PCR;对于怀疑有t(8;21)变异型、del(16)(q22)或+22的患者,也需要进行RT-PCR以确定是否为CBF AML。RT-PCR不应取代细胞遗传学,也不应作为检测CBF AML的唯一诊断试验,因为可能会出现假阳性或假阴性结果。
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