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[从动物组织中分离纯化的线粒体DNA(不含有核DNA)(甲基化程度和嘧啶核苷酸聚类水平——纯度标准)]

[Isolation of mitochondrial DNA, purified of nuclear DNA, from animal tissues (degree of methylation and level of pyrimidine nucleotide clustering--criteria of purity)].

作者信息

Kirnos M D, Vaniushin B F

出版信息

Biokhimiia. 1976 Jan;41(1):68-74.

PMID:6074
Abstract

A method of preparation of mitochondria free of nuclear DNA and its fragments by treatment of mitochondria with DEAE-cellulose has been developed. This method is based on binding nuclear nucleic acids and nucleoproteins to DEAE-cellulose particles in the media used for isolation of mitochondria. Treatment with DEAE-cellulose under the conditions described does not induce any visible degradation of mitochondria and mitochondrial DNA. The mitochondrial DNA preparations obtained from beef and rat liver are represented with closed circular molecules of contour length about 5.5 mu. The 5-methylcytosine content in beef and rat mitochondrial DNA (3.03 and 2.0 mole %, respectively) is twice as much as in corresponding nuclear DNA. Besides, mitochondrial DNA strongly differs from nuclear ones by a lower degree of pyrimidine clustering: the amount of mono- and dipyrimidine fragments (about 32 mole %) in mitochondrial DNA is 1.5 times as large and the content of long pyrimidine clusters (hexa- and others) is 2--4 times as low as those in nuclear DNA. The methylation level and the pyrimidine clustering degree may be used as criteria for the purity of mitochondrial DNA from nuclear DNA.

摘要

已开发出一种通过用二乙氨基乙基纤维素(DEAE - 纤维素)处理线粒体来制备不含核DNA及其片段的线粒体的方法。该方法基于在用于分离线粒体的培养基中,将核核酸和核蛋白与DEAE - 纤维素颗粒结合。在所描述的条件下用DEAE - 纤维素处理不会引起线粒体和线粒体DNA的任何可见降解。从牛肉和大鼠肝脏获得的线粒体DNA制剂呈现为轮廓长度约5.5微米的闭环分子。牛肉和大鼠线粒体DNA中的5 - 甲基胞嘧啶含量(分别为3.03和2.0摩尔%)是相应核DNA中的两倍。此外,线粒体DNA与核DNA的显著差异在于嘧啶聚集程度较低:线粒体DNA中单嘧啶和双嘧啶片段的量(约32摩尔%)是核DNA中的1.5倍,而长嘧啶簇(六聚体及其他)的含量比核DNA低2 - 4倍。甲基化水平和嘧啶聚集程度可作为线粒体DNA相对于核DNA纯度的标准。

相似文献

1
[Isolation of mitochondrial DNA, purified of nuclear DNA, from animal tissues (degree of methylation and level of pyrimidine nucleotide clustering--criteria of purity)].[从动物组织中分离纯化的线粒体DNA(不含有核DNA)(甲基化程度和嘧啶核苷酸聚类水平——纯度标准)]
Biokhimiia. 1976 Jan;41(1):68-74.
2
Structure of animal mitochondrial DNA: nucleotide composition, pyrimidine clusters, and methylation character.动物线粒体DNA的结构:核苷酸组成、嘧啶簇及甲基化特征
Mol Biol (Mosk). 1976 Jul-Aug;10(4):715-24.
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Structure of animal mitochondrial DNA (base composition, pyrimidine clusters, character of methylation).动物线粒体DNA的结构(碱基组成、嘧啶簇、甲基化特征)
Biochim Biophys Acta. 1977 Mar 18;475(2):323-36. doi: 10.1016/0005-2787(77)90023-5.
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[Isolation and characteristics of DNA fragments bound to mitochondrial membrane proteins].[与线粒体膜蛋白结合的DNA片段的分离及特性研究]
Mol Biol (Mosk). 1977 Sep-Oct;11(5):1029-38.
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The structure of animal mitochondrial DNA (base composition, pyrimidine clusters, character of methylation).动物线粒体DNA的结构(碱基组成、嘧啶簇、甲基化特征)
Mol Cell Biochem. 1977 Feb 4;14(1-3):31-6. doi: 10.1007/BF01734162.
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[Character of the methylation and reassociation of wheat DNA fractions differing in their nucleotide composition].[核苷酸组成不同的小麦DNA组分的甲基化和复性特征]
Mol Biol (Mosk). 1978 Jul-Aug;12(4):845-52.
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Fragmented mitochondrial DNA is the predominant carrier of oxidized DNA bases.碎片化的线粒体DNA是氧化DNA碱基的主要载体。
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[DNA-methylase activities from animal mitochondria and nuclei: different specificity of DNA methylation].[动物线粒体和细胞核中的DNA甲基化酶活性:DNA甲基化的不同特异性]
Biokhimiia. 1976 Nov;41(11):1968-77.
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[Distribution of 5-methylcytosine in pyrimidine oligonucleotides of higher plant DNA].[高等植物DNA嘧啶寡核苷酸中5-甲基胞嘧啶的分布]
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[Cytochrome oxidase of rat liver nuclear membranes and its interaction with mitochondrial cytochrome oxidase].[大鼠肝细胞核膜细胞色素氧化酶及其与线粒体细胞色素氧化酶的相互作用]
Biokhimiia. 1976 Sep;41(9):1684-97.

引用本文的文献

1
Mitochondrial DNA: Epigenetics and environment.线粒体 DNA:表观遗传学与环境。
Environ Mol Mutagen. 2019 Oct;60(8):668-682. doi: 10.1002/em.22319. Epub 2019 Aug 6.
2
CpG methylation patterns of human mitochondrial DNA.人类线粒体DNA的CpG甲基化模式
Sci Rep. 2016 Mar 21;6:23421. doi: 10.1038/srep23421.
3
The structure of animal mitochondrial DNA (base composition, pyrimidine clusters, character of methylation).动物线粒体DNA的结构(碱基组成、嘧啶簇、甲基化特征)
Mol Cell Biochem. 1977 Feb 4;14(1-3):31-6. doi: 10.1007/BF01734162.