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通过能量过滤透射电子显微镜对噬菌体内部DNA和抗衡离子含量进行化学映射分析。

Chemical mapping of DNA and counter-ion content inside phage by energy-filtered TEM.

作者信息

Nevsten Pernilla, Evilevitch Alex, Wallenberg Reine

机构信息

nCHREM, Polymer and Materials Chemistry, Kemicentrum, Lund University, P.O. Box 124, 221 00 Lund, Sweden.

出版信息

J Biol Phys. 2012 Mar;38(2):229-40. doi: 10.1007/s10867-011-9234-8. Epub 2011 Aug 26.

Abstract

Double-stranded DNA in many bacterial viruses (phage) is strongly confined, which results in internal genome pressures of tens of atmospheres. This pressure is strongly dependent on local ion concentration and distribution within the viral capsid. Here, we have used electron energy loss spectroscopy (EELS), energy-filtered TEM (EFTEM) and X-ray energy dispersive spectroscopy to provide such chemical information from the capsid and the phage tail through which DNA is injected into the cell. To achieve this, we have developed a method to prepare thin monolayers of self-supporting virus/buffer films, suitable for EELS and EFTEM analysis. The method is based on entrapment of virus particles at air-liquid interfaces; thus, the commonly used method of staining by heavy metal salts can be avoided, eliminating the risk for chemical artifacts. We found that Mg(2 + ) concentration was approximately 2-4 times higher in the DNA-filled capsid than in the surrounding TM buffer (containing 10 mM Mg(2 + )). Furthermore, we also analyzed the DNA content inside the phage tail by mapping phosphorus and magnesium.

摘要

许多细菌病毒(噬菌体)中的双链DNA受到强烈限制,这导致内部基因组压力达到数十个大气压。这种压力强烈依赖于病毒衣壳内的局部离子浓度和分布。在这里,我们使用电子能量损失谱(EELS)、能量过滤透射电子显微镜(EFTEM)和X射线能量色散谱来从衣壳和噬菌体尾部提供此类化学信息,DNA通过这些部位注入细胞。为实现这一点,我们开发了一种制备适用于EELS和EFTEM分析的自支撑病毒/缓冲液薄膜薄单层的方法。该方法基于将病毒颗粒截留在气液界面;因此,可以避免常用的重金属盐染色方法,消除化学假象的风险。我们发现,充满DNA的衣壳中的Mg(2 +)浓度比周围的TM缓冲液(含有10 mM Mg(2 +))高约2至4倍。此外,我们还通过绘制磷和镁的分布图分析了噬菌体尾部内部的DNA含量。

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