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用于流式细胞术的染色体悬液制备

Preparation of chromosome suspensions for flow cytometry.

作者信息

van den Engh G, Trask B, Cram S, Bartholdi M

出版信息

Cytometry. 1984 Mar;5(2):108-17. doi: 10.1002/cyto.990050203.

Abstract

Certain variables in the preparation of chromosome suspensions for flow cytometric analysis have been investigated. The optimal conditions have been determined. The results of this series of experiments have been incorporated to yield a preparation protocol that gives chromosome profiles with a low amount of small particle debris and few chromosome clumps. The method reduces variability that results from sample preparation. Chromosomes are optimally isolated in a hypotonic solution buffered to pH 8.0. MgSO4 and dithiothreitol added to the buffer reduce the number of clumps and small fluorescent particles. The presence of MgSO4 also stabilizes the chromosomes and precludes the need for other stabilizing agents such as propidium iodide. When the swelling buffer developed in this investigation is used, unstained chromosomes are stable for at least 1 wk if stored at 4 degrees C. The preparation procedure can be used with the DNA stains, propidium iodide, Hoechst 33258, and mithramycin. Preliminary experiments show that this procedure can also be used for bivariate analysis of human and Chinese hamster chromosomes. The importance of this improvement for studies on chromosome damage caused by irradiation or mutagens is discussed.

摘要

对用于流式细胞术分析的染色体悬浮液制备过程中的某些变量进行了研究。确定了最佳条件。结合这一系列实验的结果,得出了一种制备方案,该方案能产生小颗粒碎片少且染色体团块少的染色体图谱。该方法减少了样本制备过程中产生的变异性。染色体在缓冲至pH 8.0的低渗溶液中得到最佳分离。添加到缓冲液中的硫酸镁和二硫苏糖醇减少了团块和小荧光颗粒的数量。硫酸镁的存在还能稳定染色体,无需使用其他稳定剂,如碘化丙啶。当使用本研究中开发的膨胀缓冲液时,未染色的染色体如果保存在4℃,至少可稳定1周。该制备程序可与DNA染料碘化丙啶、Hoechst 33258和光神霉素一起使用。初步实验表明,该程序也可用于人类和中国仓鼠染色体的双变量分析。讨论了这一改进对研究辐射或诱变剂引起的染色体损伤的重要性。

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