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胶原蛋白原纤维形成的圆二色光谱:一项旧技术的新用途。

Circular Dichroism Spectroscopy of Collagen Fibrillogenesis: A New Use for an Old Technique.

作者信息

Drzewiecki Kathryn E, Grisham Daniel R, Parmar Avanish S, Nanda Vikas, Shreiber David I

机构信息

Department of Biomedical Engineering, Rutgers, The State University of New Jersey, Piscataway, New Jersey.

Department of Physics, Indian Institute of Technology, Banaras Hindu University, Varanasi, Uttar Pradesh, India.

出版信息

Biophys J. 2016 Dec 6;111(11):2377-2386. doi: 10.1016/j.bpj.2016.10.023.

Abstract

Type-I collagen assembles in a stepwise, hierarchic fashion from the folding of the triple helix to the assembly of fibrils into fibers. The mature assembled fibers are crucial for tissue structure and mechanics, cell interactions, and other functions in vivo. Although triple helix folding can be followed with the use of optical methods such as circular dichroism (CD) spectroscopy, fibrillogenesis is typically measured by alternative methods such as turbidity, rheology, and microscopy. Together, these approaches allow for investigation of the mechanical properties and architectures of collagen-based scaffolds and excised tissues. Herein, we demonstrate that CD spectroscopy, a technique that is used primarily to evaluate the secondary structure of proteins, can also be employed to monitor collagen fibrillogenesis. Type-I collagen suspensions demonstrated a strong, negative ellipticity band between 204 and 210 nm under conditions consistent with fibrillogenesis. Deconvolution of CD spectra before, during, and after fibrillogenesis identified a unique fibril spectrum distinct from triple helix and random coil conformations. The ability to monitor multiple states of collagen simultaneously in one experiment using one modality provides a powerful platform for studying this complex assembly process and the effects of other factors, such as collagenases, on fibrillogenesis and degradation.

摘要

I型胶原蛋白以逐步、分级的方式组装,从三螺旋的折叠到原纤维组装成纤维。成熟的组装纤维对于组织结构和力学、细胞相互作用以及体内的其他功能至关重要。尽管可以使用诸如圆二色性(CD)光谱等光学方法来跟踪三螺旋折叠,但原纤维形成通常通过诸如浊度、流变学和显微镜等替代方法来测量。这些方法共同使得能够研究基于胶原蛋白的支架和切除组织的力学性能和结构。在此,我们证明,主要用于评估蛋白质二级结构的CD光谱技术,也可用于监测胶原蛋白的原纤维形成。在与原纤维形成一致的条件下,I型胶原蛋白悬浮液在204至210nm之间显示出强烈的负椭圆率带。对原纤维形成之前、期间和之后的CD光谱进行去卷积,确定了一种独特的原纤维光谱,不同于三螺旋和无规卷曲构象。使用一种模式在一个实验中同时监测胶原蛋白多种状态的能力,为研究这种复杂的组装过程以及诸如胶原酶等其他因素对原纤维形成和降解的影响提供了一个强大的平台。

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