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一些健康个体血液中主要BCR-ABL的表达水平非常低。

Very low level of major BCR-ABL expression in blood of some healthy individuals.

作者信息

Biernaux C, Sels A, Huez G, Stryckmans P

机构信息

Laboratory of Biological Chemistry, Université Libre de Bruxelles, Belgium.

出版信息

Bone Marrow Transplant. 1996 May;17 Suppl 3:S45-7.

PMID:8769701
Abstract

The nested reverse transcriptase polymerase chain reaction (RT-PCR) provides a powerful tool for detection of minimal residual disease in CML. The RT-PCR used in the present study for detection of the major bcr-abl fusion gene, the hallmark and presumably the cause of CML, was optimized by: (a) increasing the amount of total RNA involved in the reverse transcription reaction to correspond to total RNA extracted from 10(8) cells; (b) using a specific abl primer in this reverse transcriptase reaction, and (c) reamplifying 10% of the RT-PCR product in a nested amplification. This optimized RT-PCR permitted to detect up to 1 copy of RNA bcr-abl synthesized in vitro, mixed with yeast RNA in a quantity equivalent to 10(8) white blood cells (WBC). Using the highly sensitive RT-PCR, a systematic study of the possible expression of bcr-abl RNA in WBC of healthy adults, children and umbilical cord blood (UCB) revealed the presence of bcr-abl transcripts in blood cells of 22/73 adults, 1/22 children but not in 22 samples of UCB. The comparison of these three groups indicated a significant tendency for the anomaly to increase in frequency with age.

摘要

巢式逆转录聚合酶链反应(RT-PCR)为检测慢性粒细胞白血病(CML)中的微小残留病提供了一种强大的工具。本研究中用于检测主要bcr-abl融合基因(CML的标志且可能是其病因)的RT-PCR通过以下方式进行了优化:(a)增加逆转录反应中所涉及的总RNA量,使其与从10⁸个细胞中提取的总RNA量相对应;(b)在该逆转录反应中使用特异性abl引物;以及(c)在巢式扩增中对10%的RT-PCR产物进行再扩增。这种优化后的RT-PCR能够检测出体外合成的低至1份与相当于10⁸个白细胞(WBC)数量的酵母RNA混合的RNA bcr-abl。使用高度灵敏的RT-PCR,对健康成人、儿童及脐带血(UCB)白细胞中bcr-abl RNA的可能表达进行的系统研究显示,在73名成人中的22名、22名儿童中的1名的血细胞中存在bcr-abl转录本,但在22份UCB样本中未检测到。这三组的比较表明,该异常的频率有随年龄增加而显著上升的趋势。

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