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Application of a modified drop method for high-resolution pachytene chromosome spreads in two Phalaenopsis species

机译:改性液滴法在两种鳞片肌染色体中的应用

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Preparation of good chromosome spreads without cytoplasmic contamination is the crucial step in cytogenetic mapping. To date, cytogenetic research in the Orchidaceae family has been carried out solely on mitotic metaphase chromosomes. Well-spread meiotic pachytene chromosomes can provide higher resolution and fine detail for analysis of chromosomal structure and are also beneficial for chromosomal FISH (fluorescence in situ hybridization) mapping. However, an adequate method for the preparation of meiotic pachytene chromosomes in orchid species has not yet been reported. Two Taiwanese native Phalaenopsis species were selected to test the modified drop method for preparation of meiotic pachytene chromosomes from pollinia. In this modified method, pollinia were ground and treated with an enzyme mixture to completely remove cell walls. Protoplasts were resuspended in ethanol/glacial acetic acid and dropped onto a wet inclined slide of 30° from a height of 0.5?m. The sample was then flowed down the inclined plane to spread the chromosomes. Hundreds of pachytene chromosomes with little to no cytoplasmic contamination were well spread on each slide. We also showed that the resolution of 45S rDNA-containing chromosomes at the pachytene stage was up to 20 times higher than that at metaphase. Slides prepared following this modified drop method were amenable to FISH mapping of both 45S and 5S rDNA on pachytene chromosomes and, after FISH, the chromosomal structure remained intact for further analysis. This modified drop method is suitable for pachytene spreads from pollinia of Phalaenopsis orchids. The large number and high-resolution pachytene spreads, with little or no cytoplasmic contamination, prepared by the modified drop method could be used for FISH mapping of DNA fragments to accelerate the integration of cytogenetic and molecular research in Phalaenopsis orchids.
机译:没有细胞质污染的良好染色体污染的制备是细胞遗传学映射的关键步骤。迄今为止,兰科西族的细胞遗传学研究仅在有丝分裂中期染色体上进行。良好的减少的减少的嗜酚肽染色体可以提供更高的分辨率和细节,用于分析染色体结构,也是有益于染色体鱼(荧光原位杂交)测绘。然而,尚未报告兰花物种中制备减数分裂性噬菌体染色体的足够方法。选择两种台湾天然植入蝴蝶兰类物种以测试从Pollinia制备染色体磷酸染色体的改性液滴方法。在这种改性方法中,用酶混合物研磨并用酶混合物处理,以完全去除细胞壁。将原生质体重悬于乙醇/冰醋酸中,并将其掉在30°的湿倾斜载玻片上,从0.5μm的高度掉。然后将样品流下倾斜平面以扩散染色体。数百种没有细胞质污染的嗜孢子染色体在每个载玻片上均匀蔓延。我们还表明,含有45秒的含有45s含有RDNA染色体的分辨率高达比中期的20倍。在这种改进的液滴法制下制备的载玻片均可用于在慢性染色体上的45s和5s rdNA的鱼类测绘,并且在鱼之后,染色体结构保持完整,用于进一步分析。这种改性的液滴方法适用于兰彭斯兰花的POLLINIA的嗜孢子酱。通过修饰的液滴方法制备的大量和高分辨率噬藻丁烯蔓延,几乎没有细胞质污染,可用于DNA片段的鱼类映射,以加速细胞遗传学和分子研究在兰花植物兰花中的整合。

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