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用碳和氮标记淀粉样β蛋白和抑制性肽,通过纳米级红外光谱研究它们的相互作用。

C- and N-labeling of amyloid-β and inhibitory peptides to study their interaction via nanoscale infrared spectroscopy.

作者信息

Paul Suman, Jeništová Adéla, Vosough Faraz, Berntsson Elina, Mörman Cecilia, Jarvet Jüri, Gräslund Astrid, Wärmländer Sebastian K T S, Barth Andreas

机构信息

Department of Biochemistry and Biophysics, Stockholm University, Stockholm, Sweden.

attocube systems AG, Haar, Germany.

出版信息

Commun Chem. 2023 Aug 3;6(1):163. doi: 10.1038/s42004-023-00955-w.

Abstract

Interactions between molecules are fundamental in biology. They occur also between amyloidogenic peptides or proteins that are associated with different amyloid diseases, which makes it important to study the mutual influence of two polypeptides on each other's properties in mixed samples. However, addressing this research question with imaging techniques faces the challenge to distinguish different polypeptides without adding artificial probes for detection. Here, we show that nanoscale infrared spectroscopy in combination with C, N-labeling solves this problem. We studied aggregated amyloid-β peptide (Aβ) and its interaction with an inhibitory peptide (NCAM1-PrP) using scattering-type scanning near-field optical microscopy. Although having similar secondary structure, labeled and unlabeled peptides could be distinguished by comparing optical phase images taken at wavenumbers characteristic for either the labeled or the unlabeled peptide. NCAM1-PrP seems to be able to associate with or to dissolve existing Aβ fibrils because pure Aβ fibrils were not detected after mixing.

摘要

分子间相互作用是生物学的基础。这种相互作用也发生在与不同淀粉样疾病相关的淀粉样生成肽或蛋白质之间,这使得研究混合样品中两种多肽对彼此性质的相互影响变得很重要。然而,用成像技术解决这个研究问题面临着在不添加人工检测探针的情况下区分不同多肽的挑战。在这里,我们表明,结合碳、氮标记的纳米级红外光谱解决了这个问题。我们使用散射型扫描近场光学显微镜研究了聚集的淀粉样β肽(Aβ)及其与抑制肽(NCAM1-PrP)的相互作用。尽管标记和未标记的肽具有相似的二级结构,但通过比较在标记或未标记肽的特征波数下拍摄的光学相位图像,可以区分它们。NCAM1-PrP似乎能够与现有的Aβ纤维结合或溶解它们,因为混合后未检测到纯Aβ纤维。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e224/10400569/6f7526e30a2e/42004_2023_955_Fig1_HTML.jpg

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