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通过二次离子质谱法进行具有高横向分辨率的支撑膜成分分析。

Supported membrane composition analysis by secondary ion mass spectrometry with high lateral resolution.

作者信息

Galli Marxer Carine, Kraft Mary L, Weber Peter K, Hutcheon Ian D, Boxer Steven G

机构信息

Department of Chemistry, Stanford University, Stanford, California 94305, USA.

出版信息

Biophys J. 2005 Apr;88(4):2965-75. doi: 10.1529/biophysj.104.057257. Epub 2005 Feb 4.

Abstract

The lateral organization of lipid components within membranes is usually investigated with fluorescence microscopy, which, though highly sensitive, introduces bulky fluorophores that might alter the behavior of the components they label. Secondary ion mass spectroscopy performed with a NanoSIMS 50 instrument also provides high lateral resolution and sensitivity, and many species can be observed in parallel without the use of bulky labels. A tightly focused beam (approximately 100 nm) of Cs ions is scanned across a sample, and up to five of the resulting small negative secondary ions can be simultaneously analyzed by a high-resolution mass spectrometer. Thin layers of (15)N- and (19)F-labeled proteins were microcontact-printed on an oxidized silicon substrate and imaged using the NanoSIMS 50, demonstrating the sensitivity and selectivity of this approach. Supported lipid bilayers were assembled on an oxidized silicon substrate, then flash-frozen and freeze-dried to preserve their lateral organization. Lipid bilayers were analyzed with the NanoSIMS 50, where the identity of each specific lipid was determined through detection of its unique secondary ions, including (12)C(1)H(-), (12)C(2)H(-), (13)C(-), (12)C(14)N(-), and (12)C(15)N(-). Steps toward obtaining quantitative composition analysis of lipid membranes that varied spatially in isotopic composition are presented. This approach has the potential to provide a composition-specific analysis of membrane organization that compliments other imaging modalities.

摘要

膜内脂质成分的侧向组织通常用荧光显微镜进行研究,这种方法虽然高度灵敏,但会引入体积较大的荧光团,可能会改变它们所标记成分的行为。用NanoSIMS 50仪器进行的二次离子质谱分析也具有高侧向分辨率和灵敏度,并且无需使用体积较大的标记物就能同时观察多种物质。一束聚焦紧密(约100纳米)的铯离子束扫描样品,产生的多达五个小的负二次离子可由高分辨率质谱仪同时分析。将(15)N和(19)F标记的蛋白质薄层通过微接触印刷法印在氧化硅衬底上,并用NanoSIMS 50成像,证明了这种方法的灵敏度和选择性。在氧化硅衬底上组装支持脂质双层,然后快速冷冻和冻干以保持其侧向组织。用NanoSIMS 50分析脂质双层,通过检测其独特的二次离子(包括(12)C(1)H(-)、(12)C(2)H(-)、(13)C(-)、(12)C(14)N(-)和(12)C(15)N(-))来确定每种特定脂质的身份。本文介绍了对同位素组成在空间上变化的脂质膜进行定量组成分析的步骤。这种方法有可能提供对膜组织的成分特异性分析,以补充其他成像方式。

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