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首页> 外文期刊>Experimental Hematology: Official Publication of the International Society for Experimental Hematology >Cyclin D1 (CCND1) messenger RNA expression as assessed by real-time PCR contributes to diagnosis and follow-up control in patients with mantle cell lymphoma
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Cyclin D1 (CCND1) messenger RNA expression as assessed by real-time PCR contributes to diagnosis and follow-up control in patients with mantle cell lymphoma

机译:实时荧光定量PCR评估细胞周期蛋白D1(CCND1)信使RNA的表达有助于诊断和随访控制套细胞淋巴瘤患者

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Molecular diagnosis of mantle cell lymphoma (MCL) can be difficult because the t(11;14)/IGH@-CCND1 is extremely heterogeneous at the DNA level. Aiming to establish a reliable molecular tool that could be easily implemented in routine diagnostics, we developed a new real-time polymerase chain reaction (PCR) assay for CCND1 expression measurement and evaluated 451 cases: 142 MCL, 76 chronic lymphocytic leukemia, 20 hairy cell leukemia, 13 hairy cell leukemia-variant, 20 splenic marginal zone lymphoma, 91 other mature B-cell neoplasms, 29 other hematologic neoplasms, and 60 healthy individuals. Sensitivity of the real-time PCR assay was up to 10-4. In t(11;14)/IGH@-CCND1 positive lymphoma samples (n= 150), median %CCND1/ABL1 expression level was 178.2 (range: 1.5-4, 152.0). Normalized by t(11;14)/IGH@-CCND1 positive cells as determined by fluorescence in situ hybridization IGH@-CCND1 positive samples showed a median %CCND1/ABL1 of 445.8 (range: 17.9-4,848.5). A normalized %CCND1/ABL1 expression of at least 17.0 was chosen as threshold for CCND1 positivity. For unnormalized samples, the positive detection rate oft(11;14)/IGH@-CCND1 by CCND1 expression was 87.3%. Healthy individuals had low%CCND1/ABL1 (median, 1.1; range, 0.0-7.8). The negative predictive value for exclusionof a t(11;14)/IGH@-CCND1 by CCND1 expression was 95.3% by the above threshold. %CCND1/ABL1 was higher in MCL than in the remaining B-cell lymphomas (mean ± SD, 392.9 ± 685.3 vs. 46.0 ± 305.0; p 0.001). In 66 follow-up samples, CCND1 showed 2.5-3.5 log reduction after chemotherapy and increase at relapse. CCND1 expression could serve as adjunct to other techniques in diagnosis and follow-up of B-cell lymphomas.
机译:外套细胞淋巴瘤(MCL)的分子诊断可能很困难,因为t(11; 14)/ IGH @ -CCND1在DNA水平上极为不同。为了建立一种可以在常规诊断中轻松实施的可靠分子工具,我们开发了一种用于CCND1表达测量的新型实时聚合酶链反应(PCR)检测方法,并评估了451例病例:142例MCL,76例慢性淋巴细胞性白血病,20例毛细胞白血病,13例毛细胞白血病变异型,20例脾边缘区淋巴瘤,91例其他成熟的B细胞肿瘤,29例其他血液学肿瘤和60例健康个体。实时PCR检测的灵敏度高达10-4。在t(11; 14)/ IGH @ -CCND1阳性淋巴瘤样本(n = 150)中,%CCND1 / ABL1表达水平的中位数为178.2(范围:1.5-4、152.0)。通过荧光原位杂交确定的t(11; 14)/ IGH @ -CCND1阳性细胞进行归一化IGH @ -CCND1阳性样品显示中位%CCND1 / ABL1为445.8(范围:17.9-4,848.5)。选择至少17.0的标准化%CCND1 / ABL1表达作为CCND1阳性的阈值。对于未归一化的样品,通过CCND1表达的t(11; 14)/ IGH @ -CCND1的阳性检出率为87.3%。健康个体的CCND1 / ABL1%低(中位数为1.1;范围为0.0-7.8)。通过上述阈值排除通过CCND1表达排除t(11; 14)/ IGH @ -CCND1的阴性预测值为95.3%。 MCL中的%CCND1 / ABL1高于其余B细胞淋巴瘤(平均值±SD,392.9±685.3 vs. 46.0±305.0; p <0.001)。在66个随访样本中,CCND1在化疗后显示2.5-3.5 log的减少,在复发时增加。 CCND1表达可以作为其他技术辅助B细胞淋巴瘤的诊断和随访。

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