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核酸可编程蛋白质阵列:用于基于阵列的功能性蛋白质研究的多功能工具。

Nucleic Acid programmable protein arrays: versatile tools for array-based functional protein studies.

作者信息

Miersch Shane, LaBaer Joshua

机构信息

Biodesign Institute at Arizona State University, Tempe, Arizona.

出版信息

Curr Protoc Protein Sci. 2011 Apr;Chapter 27:Unit27.2. doi: 10.1002/0471140864.ps2702s64.

DOI:10.1002/0471140864.ps2702s64
PMID:21488044
Abstract

Protein microarrays offer a global perspective on the function of expressed gene products. However, technical issues related to the stability and dynamic range of microarrays printed with purified protein have hampered their widespread adoption. Taking an alternate approach, the Nucleic Acid Programmable Protein Array (NAPPA) is constructed by spotting protein-encoding plasmid DNA at high density, in addressable fashion, on an array surface. Proteins are subsequently generated in situ just prior to experimentation using cell-free expression systems. As such, the NAPPA platform offers a unique and viable alternative that circumvents many of the inherent limitations of spotted protein arrays, enabling diverse functional protein studies including protein-small molecule, protein-protein, antigen-antibody, and protein-nucleic acid interactions. It further offers a versatile and adaptable platform amenable to a variety of capture modalities and expression systems, and, most importantly, construction of the array is accessible to any lab with an array printer and laser slide scanner. This unit is intended to provide a reference for investigators wishing to generate arrays based on this platform, and details (1) the basic construction of cDNA-based protein microarrays from DNA isolation to printing and development, (2) quality-control efforts taken to ensure the usefulness and integrity of microarray data, and (3) a particular example of the application of self-assembling protein arrays to screen for blood-borne antibody biomarkers.

摘要

蛋白质微阵列可全面了解已表达基因产物的功能。然而,与纯化蛋白质打印微阵列的稳定性和动态范围相关的技术问题阻碍了它们的广泛应用。采用另一种方法,核酸可编程蛋白质阵列(NAPPA)是通过将编码蛋白质的质粒DNA以高密度、可寻址的方式点样在阵列表面构建而成的。随后,在实验前使用无细胞表达系统在原位生成蛋白质。因此,NAPPA平台提供了一种独特且可行的替代方案,规避了斑点蛋白质阵列的许多固有局限性,能够进行包括蛋白质 - 小分子、蛋白质 - 蛋白质、抗原 - 抗体和蛋白质 - 核酸相互作用在内的多种功能蛋白质研究。它还提供了一个通用且适应性强的平台,适用于各种捕获方式和表达系统,最重要的是,任何拥有阵列打印机和激光载玻片扫描仪的实验室都可以构建该阵列。本单元旨在为希望基于此平台生成阵列的研究人员提供参考,并详细介绍(1)从DNA分离到打印和显影的基于cDNA的蛋白质微阵列的基本构建方法,(2)为确保微阵列数据的有用性和完整性所采取的质量控制措施,以及(3)自组装蛋白质阵列用于筛选血源抗体生物标志物的具体应用示例。

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