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gDNA qPCR is statistically more reliable than mRNA analysis in detecting leukemic cells to monitor CML

机译:在检测白血病细胞以监测CML方面,gDNA qPCR在统计上比mRNA分析更可靠

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摘要

Chronic Myeloid Leukemia (CML) is a stem cell cancer that arises when t(9;22) translocation occurs in a hematopoietic stem cells. This event results in the expression of the BCR-ABL1 fusion gene, which codes for a constitutively active tyrosine kinase that is responsible for the transformation of a HSC into a CML stem cell, which then gives rise to a clonal myeloproliferative disease. The introduction of Tyrosine Kinase Inhibitors (TKIs) has revolutionized the management of the disease. However, these drugs do not seem to be able to eradicate the malignancy. Indeed, discontinuation trials (STIM; TWISER; DADI) for those patients who achieved a profound molecular response showed 50% relapsing within 12 months. We performed a comparative analysis on 15 CML patients and one B-ALL patient, between the standard quantitative reverse-transcriptase PCR (qRT–PCR) and our genomic DNA patient-specific quantitative PCR assay (gDNA qPCR). Here we demonstrate that gDNA qPCR is better than standard qRT–PCR in disease monitoring after an average follow-up period of 200 days. Specifically, we statistically demonstrated that DNA negativity is more reliable than RNA negativity in indicating when TKIs therapy can be safely stopped.
机译:慢性粒细胞白血病(CML)是干细胞癌,当造血干细胞中发生t(9; 22)易位时会发生。此事件导致BCR-ABL1融合基因的表达,该基因编码组成性活性酪氨酸激酶,该酪氨酸激酶负责将HSC转化为CML干细胞,然后引起克隆性骨髓增生性疾病。酪氨酸激酶抑制剂(TKIs)的引入彻底改变了疾病的治疗方法。但是,这些药物似乎无法根除恶性肿瘤。确实,对于那些获得深刻分子应答的患者,终止试验(STIM; TWISER; DADI)显示在12个月内复发了50%。我们对15名CML患者和1名B-ALL患者进行了标准定量逆转录酶PCR(qRT–PCR)和我们的基因组DNA患者特异性定量PCR分析(gDNA qPCR)之间的比较分析。在这里,我们证明在平均200天的随访期之后,gDNA qPCR在疾病监测中优于标准qRT-PCR。具体而言,我们统计表明在指示何时可以安全停止TKIs治疗时,DNA阴性比RNA阴性更可靠。

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