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多重印章转移原子力显微镜沉积提高了蛋白质 - DNA构象状态的分辨率。

Multiplexed stamp-transfer AFM deposition improves resolution of protein-DNA conformational states.

作者信息

Lentz Emily, Li Zimeng, Davis Corey, Erie Dorothy A

机构信息

Department of Chemistry, University of North Carolina, Chapel Hill, North Carolina.

Department of Chemistry, University of North Carolina, Chapel Hill, North Carolina; Lineberger Comprehensive Cancer Center, University of North Carolina, Chapel Hill, North Carolina.

出版信息

Biophys J. 2025 Aug 5;124(15):2488-2499. doi: 10.1016/j.bpj.2025.06.027. Epub 2025 Jun 25.

DOI:10.1016/j.bpj.2025.06.027
PMID:40566679
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12333928/
Abstract

Single-molecule analysis of atomic force microscopy (AFM) images is a powerful tool for characterizing the structural and conformational properties of proteins, DNA, and protein-DNA complexes, as well as nonbiological molecules, such as polymers. Since the invention of AFM in 1986, significant technical advances have been made, including faster scan speeds and automated image collection and analysis. Deposition methods, however, remain essentially unchanged. Typically, several microliters of the sample are dropped onto a mica surface (unmodified or modified), allowed to spread, rinsed with water, and dried. Although this method is generally effective, it remains a chokepoint to efficiently collecting AFM data. To alleviate this bottleneck, we invented a stamp-transfer method to deposit multiple samples simultaneously onto a mica surface for imaging. We fabricate arrays of microwells in a silicon chip, fill them with samples, and bring the silicon chip into soft contact with mica to transfer the sample. This method not only allows the simultaneous deposition of multiple different protein and DNA samples, but it also expands the buffer conditions for deposition of DNA and protein-DNA complexes onto an unmodified the mica surface into the physiological salt range. Furthermore, our data indicate that the stamp-transfer deposition significantly improves the ability to resolve different conformational states of protein-DNA complexes from one another. Finally, this method can be readily automated and has the potential revolutionize AFM imaging both by improving resolution and making it "high throughput."

摘要

原子力显微镜(AFM)图像的单分子分析是一种强大的工具,可用于表征蛋白质、DNA、蛋白质-DNA复合物以及非生物分子(如聚合物)的结构和构象特性。自1986年AFM发明以来,已取得了重大技术进步,包括更快的扫描速度以及自动图像采集和分析。然而,沉积方法基本上仍未改变。通常,将几微升样品滴到云母表面(未修饰或已修饰),使其扩散,用水冲洗,然后干燥。尽管这种方法通常是有效的,但它仍然是有效收集AFM数据的一个瓶颈。为了缓解这一瓶颈,我们发明了一种印章转移方法,可将多个样品同时沉积到云母表面进行成像。我们在硅芯片中制造微孔阵列,将样品填充到微孔中,然后使硅芯片与云母软接触以转移样品。这种方法不仅允许同时沉积多个不同的蛋白质和DNA样品,而且还将DNA和蛋白质-DNA复合物沉积到未修饰云母表面的缓冲条件扩展到生理盐范围。此外,我们的数据表明,印章转移沉积显著提高了分辨蛋白质-DNA复合物不同构象状态的能力。最后,这种方法可以很容易地实现自动化,并且有潜力通过提高分辨率并使其“高通量”来彻底改变AFM成像。

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