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一种用于急性淋巴细胞白血病的直接骨髓染色体技术。

A direct bone marrow chromosome technique for acute lymphoblastic leukemia.

作者信息

Williams D L, Harris A, Williams K J, Brosius M J, Lemonds W

出版信息

Cancer Genet Cytogenet. 1984 Nov;13(3):239-57. doi: 10.1016/0165-4608(84)90046-3.

Abstract

We describe a direct bone marrow chromosome technique that was developed especially for use in studies of acute lymphoblastic leukemia (ALL). The features responsible for technical improvements include: the use of RPMI 1640 medium, supplemented with 30% fetal calf serum, to support cellular activity during both specimen transport and Colcemid treatment; the processing of only 0.1 ml of sedimented cells or less per centrifuge tube; the exposure of cells to Colcemid for a maximum of 25 min; control of the total time of exposure to hypotonic solution; the use of a steel wire as a stirring rod (fashioned to fit the centrifuge tube) for mixing cells; slide preparation by a specific edging-flaming technique; the natural aging of the slides to achieve optimal drying; and the use of a modified G-banding procedure that employs Wright's stain. This technique has been used in more than 350 cases of ALL and has consistently provided analyzable banded chromosomes, even in hyperdiploid cases with up to 91 chromosomes. It makes the previously recognized morphological difference between metaphases of residual normal cells and those from the leukemic clone less apparent. The edging-flaming technique of slide preparation is the most important component and is especially appropriate for spreading large numbers of chromosomes in ALL.

摘要

我们描述了一种专门为急性淋巴细胞白血病(ALL)研究开发的直接骨髓染色体技术。技术改进的特点包括:使用添加30%胎牛血清的RPMI 1640培养基,以在标本运输和秋水仙酰胺处理期间支持细胞活性;每个离心管仅处理0.1 ml或更少的沉淀细胞;细胞暴露于秋水仙酰胺的时间最长为25分钟;控制低渗溶液的总暴露时间;使用钢丝作为搅拌棒(制作成适合离心管的形状)来混合细胞;通过特定的边缘火焰技术制备玻片;玻片自然老化以实现最佳干燥;以及使用采用瑞氏染色的改良G显带程序。该技术已用于350多例ALL病例,即使在具有多达91条染色体的超二倍体病例中,也始终能提供可分析的带型染色体。它使先前公认的残留正常细胞中期与白血病克隆中期之间的形态学差异变得不那么明显。玻片制备的边缘火焰技术是最重要的组成部分,特别适合在ALL中铺展大量染色体。

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