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来自迈阿密地铁动物园的脊椎动物的DNA指数、基因组大小和电子核体积。

DNA index, genome size, and electronic nuclear volume of vertebrates from the Miami Metro Zoo.

作者信息

Krishan Awtar, Dandekar Payal, Nathan Nirmal, Hamelik Ronald, Miller Christine, Shaw Jackie

机构信息

Division of Experimental Therapeutics (R-71), Department of Radiation Oncology, University of Miami School of Medicine, Miami, Florida 33101, USA.

出版信息

Cytometry A. 2005 May;65(1):26-34. doi: 10.1002/cyto.a.20130.

Abstract

BACKGROUND

Flow cytometry is a rapid and reliable method for measuring nuclear DNA content and genome size. Fluorochrome binding characteristics, sample preparation and differences in DNA condensation, and availability of binding sites can cause variations in results obtained.

METHODS

Blood samples from 82 vertebrate species were collected in 10% dimethyl sulfoxide and stained with propidium iodide/hypotonic citrate or 4,6-diamidino-2-phenylindole dihydrochloride for analysis of DNA content and electronic nuclear volume (ENV). Trout red blood cells (TRBCs), human peripheral blood lymphocytes, and human buccal cavity cells were used as internal standards.

RESULTS

Mean fluorescence channel (MFC) values of TRBC and buccal cavity cells used as internal standards were stable at 15 to 120 min of propidium iodide staining. TRBCs mixed with other cells especially human peripheral blood cells showed an increase in MFC. ENV and MCF values were less variable in different species of birds than in reptiles or mammals. Genome size based on use of buccal cavity cells as the internal standard showed a high degree of correlation with previous reports.

CONCLUSIONS

Proper selection and use of internal standards and sample preparation are essential for reliable determination of DNA content and genome size in vertebrates by flow cytometry.

摘要

背景

流式细胞术是一种用于测量核DNA含量和基因组大小的快速且可靠的方法。荧光染料结合特性、样本制备以及DNA凝聚差异和结合位点的可用性会导致所得结果出现差异。

方法

将来自82种脊椎动物的血液样本收集于10%二甲基亚砜中,并用碘化丙啶/低渗柠檬酸盐或4,6-二脒基-2-苯基吲哚二盐酸盐染色,以分析DNA含量和电子核体积(ENV)。虹鳟红细胞(TRBC)、人外周血淋巴细胞和人颊腔细胞用作内标。

结果

用作内标的TRBC和颊腔细胞的平均荧光通道(MFC)值在碘化丙啶染色15至120分钟时保持稳定。TRBC与其他细胞(尤其是人外周血细胞)混合时,MFC会增加。不同鸟类的ENV和MCF值变化比爬行动物或哺乳动物小。以颊腔细胞作为内标计算的基因组大小与先前报告显示出高度相关性。

结论

正确选择和使用内标以及样本制备对于通过流式细胞术可靠测定脊椎动物的DNA含量和基因组大小至关重要。

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