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通过高效液相色谱法对组蛋白进行分级分离。

Histone fractionation by high-performance liquid chromatography.

作者信息

Gurley L R, Valdez J G, Prentice D A, Spall W D

出版信息

Anal Biochem. 1983 Feb 15;129(1):132-44. doi: 10.1016/0003-2697(83)90061-1.

Abstract

A method for the rapid chromatography of histones by high-performance liquid chromatography (HPLC) using a reverse-phase mu Bondapak C18 column containing a packing of octadecylsilane chemically bonded to silica and a linear elution gradient running from water to acetonitrile is described. Two conditions were found to be necessary to achieve histone fractionation: (i) silylation of the active groups of the silica solid support, and (ii) trifluoroacetic acid (TFA) in the eluting solvents. Greater than 90% of the total [3H]lysine-labeled protein applied to the column was eluted from the column. The fractionation of the histones appears to be based on the hydrophobic properties of the proteins. The HPLC histone fractions (identified by their electrophoretic mobilities) were eluted from the column in the following order: H1, H2B, (LHP)H2A, (MHP)H2A + H4, (LHP)H3, and (MHP)H3 (where LHP and MHP refer to the less hydrophobic and more hydrophobic histone variants). Phosphorylated histone species were not resolved from their unmodified parental species. The volatile nature of the water/acetonitrile/TFA eluting solvent facilitated the recovery of salt-free histones from the eluted HPLC fractions by simple lyophilization. This system is very useful for the rapid isolation of the lysine-rich histones, H1 and H2B, and the variants of histone H3. With further development, this system is expected to extend the advantages of HPLC to the fractionation of histone H4 and the variants of histone H2A as well.

摘要

描述了一种通过高效液相色谱(HPLC)快速色谱分离组蛋白的方法,该方法使用含有化学键合到硅胶上的十八烷基硅烷填料的反相μ Bondapak C18柱以及从水到乙腈的线性洗脱梯度。发现实现组蛋白分级分离需要两个条件:(i)硅胶固体支持物活性基团的硅烷化,以及(ii)洗脱溶剂中的三氟乙酸(TFA)。应用于柱的总[3H]赖氨酸标记蛋白中超过90%从柱中洗脱出来。组蛋白的分级分离似乎基于蛋白质的疏水特性。HPLC组蛋白级分(通过其电泳迁移率鉴定)按以下顺序从柱中洗脱:H1、H2B、(LHP)H2A、(MHP)H2A + H4、(LHP)H3和(MHP)H3(其中LHP和MHP分别指疏水性较低和较高的组蛋白变体)。磷酸化的组蛋白种类与其未修饰的亲本种类无法区分。水/乙腈/TFA洗脱溶剂的挥发性有助于通过简单冻干从洗脱的HPLC级分中回收无盐组蛋白。该系统对于快速分离富含赖氨酸的组蛋白H1和H2B以及组蛋白H3的变体非常有用。随着进一步发展,预计该系统也将把HPLC的优势扩展到组蛋白H4和组蛋白H2A变体的分级分离。

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