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使用数字液滴聚合酶链反应对BCR::ABL1的T315I突变进行定量检测。

Quantitative detection of T315I mutations of BCR::ABL1 using digital droplet polymerase chain reaction.

作者信息

Mu Huijun, Zou Jian, Zhang Haiping

机构信息

Department of Clinical Laboratory, the Affiliated Wuxi People's Hospital of Nanjing Medical University, Wuxi, PR China.

Department of Dermatology, Wuxi No.2 People's Hospital, Jiangnan University Medical Center, Wuxi, PR China.

出版信息

Hematol Transfus Cell Ther. 2024 Dec;46 Suppl 6(Suppl 6):S79-S85. doi: 10.1016/j.htct.2023.12.007. Epub 2024 Feb 17.

Abstract

BACKGROUND

T315I mutations of the BCR::ABL1 gene lead to resistance to tyrosine kinase inhibitors (TKIs). This study evaluated the performance of digital droplet polymerase chain reaction (ddPCR) in quantifying T315I mutations and their frequency in Philadelphia chromosome (Ph) positive hematological patients.

METHODS

The course of disease and BCR::ABL1 fusion transcripts (e13a2, e14a2 and e1a2) were retrospectively reviewed in 21 patients with acute lymphoblastic leukemia (ALL) and 85 patients with chronic myeloid leukemia (CML). T315I mutation analysis was carried out using ddPCR and the limit of detection was assessed using mutant T315I DNA at varying variant allele fractions.

RESULTS

T315I mutations were found in two ALL patients and one CML patient without remission in molecular biology and with mutation burdens of 29.20%, 40.85%, and 3.00%, respectively. The mutation burden of ALL patients was higher than that of CML patients, but there was no significant difference between the two (p-value = 0.0536). The test's limit of detection was 0.02% with a correlation coefficient greater than 0.99 between the expected and actual detection abundances.

CONCLUSION

T315I mutations have a high incidence in Ph-positive ALL patients even if the course of disease is short. In molecular biology, T315I mutation detection is indicated for CML patients not in remission.

摘要

背景

BCR::ABL1基因的T315I突变导致对酪氨酸激酶抑制剂(TKIs)耐药。本研究评估了数字液滴聚合酶链反应(ddPCR)在定量T315I突变及其在费城染色体(Ph)阳性血液病患者中的频率方面的性能。

方法

回顾性分析21例急性淋巴细胞白血病(ALL)患者和85例慢性髓性白血病(CML)患者的疾病进程及BCR::ABL1融合转录本(e13a2、e14a2和e1a2)。使用ddPCR进行T315I突变分析,并使用不同变异等位基因分数的突变型T315I DNA评估检测限。

结果

在两名ALL患者和一名CML患者中发现T315I突变,这些患者分子生物学未缓解,突变负担分别为29.20%、40.85%和3.00%。ALL患者的突变负担高于CML患者,但两者之间无显著差异(p值 = 0.0536)。该检测的检测限为0.02%,预期检测丰度与实际检测丰度之间的相关系数大于0.99。

结论

即使病程较短,T315I突变在Ph阳性ALL患者中的发生率也较高。在分子生物学方面,对于未缓解的CML患者,建议进行T315I突变检测。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1391/11726099/e4ad656a3120/gr1.jpg

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