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利用DNA嵌入剂稳定染色体用于流式核型分析及通过分离染色体显带进行鉴定。

Stabilization of chromosomes by DNA intercalators for flow karyotyping and identification by banding of isolated chromosomes.

作者信息

Aten J A, Buys C H, van der Veen A Y, Mesa J R, Yu L C, Gray J W, Osinga J, Stap J

机构信息

Laboratory for Radiobiology, University of Amsterdam, The Netherlands.

出版信息

Histochemistry. 1987;87(4):359-66. doi: 10.1007/BF00492590.

Abstract

A number of structurally unrelated DNA intercalators have been studied as stabilizers of mitotic chromosomes during isolation from rodent and human metaphase cells. Seven out of the nine intercalators tested were found to be useful as chromosome stabilizing agents. Chromosome suspensions prepared in this way could be preserved for long periods of time. After isolation the chromosomal DNA was longer than 150 kb. With intercalated chromosomes high resolution flow karyotypes could be obtained as illustrated for the non-fluorescent intercalators 9-methylene-(1,3-dimethyl-2,4-dionepyrimidine-5-yl)-phenanthrid in iumchloride and 4'-aminomethyl-4,5', 8-trimethylpsoralen combined with DAPI and 33258 Hoeschst for fluorescent staining and for the fluorescent intercalator propidium iodide used as a stabilizer and as a fluorochrome. Passage of the intercalated chromosomes through the laser beam had no measurable effect on the length of the chromosomal DNA subsequently isolated. After flow analysis and collection on slides human chromosomes could easily be banded by Giemsa staining methods with the same resolution as obtained in conventional metaphase spreads. This allowed a ready identification of about 80 percent of all chromosomes in the unfractionated suspension collected after passage through the laser beam.

摘要

许多结构不相关的DNA嵌入剂已被研究作为从啮齿动物和人类中期细胞中分离有丝分裂染色体时的稳定剂。在所测试的9种嵌入剂中,有7种被发现可作为染色体稳定剂。以这种方式制备的染色体悬浮液可以长时间保存。分离后,染色体DNA长度超过150 kb。对于嵌入的染色体,可以获得高分辨率的流式核型,如非荧光嵌入剂氯化9-亚甲基-(1,3-二甲基-2,4-二氧嘧啶-5-基)-菲啶和4'-氨甲基-4,5',8-三甲基补骨脂素与DAPI和33258 Hoechst结合用于荧光染色,以及荧光嵌入剂碘化丙啶用作稳定剂和荧光染料的情况所示。嵌入的染色体通过激光束对随后分离的染色体DNA长度没有可测量的影响。经过流式分析并收集在载玻片上后,人类染色体可以很容易地通过吉姆萨染色方法进行显带,分辨率与传统中期铺片相同。这使得在通过激光束后收集的未分级悬浮液中,约80%的所有染色体能够被轻易识别。

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