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圆二色光谱仪用于肽和蛋白质二级结构及三级结构测定的综合指南。

A comprehensive guide for secondary structure and tertiary structure determination in peptides and proteins by circular dichroism spectrometer.

作者信息

Kuril Akhilesh Kumar, Vashi Ankur, Subbappa Praveen Kumar

机构信息

Bhagwant University, Ajmer, Rajasthan, India.

Flamma USA LLC, Malvern, PA, USA.

出版信息

J Pept Sci. 2025 Jan;31(1):e3648. doi: 10.1002/psc.3648. Epub 2024 Aug 12.

DOI:10.1002/psc.3648
PMID:39135381
Abstract

Secondary structure refers to highly regular local sub-structures formed by the polypeptide backbone through hydrogen bonding. The two main types of secondary structures are α-helices and β-strands (which can form β-sheets). The development of a robust circular dichroism (CD) method for structural analysis of biomolecules requires careful consideration of several key factors. Solvent selection plays a crucial role in maintaining the native or desired conformation of the sample while ensuring transparency in the relevant wavelength regions. Aqueous buffers are often preferred for studying proteins in their native state. Optimizing the sample concentration and path length is essential to achieve an optimal absorbance range and maximize the signal-to-noise ratio. Typical concentrations for far-UV CD measurements range from 0.1 to 1 mg/ml, with shorter path lengths (1 mm) allowing for higher concentrations and longer path lengths (5 mm) suitable for dilute solutions. Instrumental parameters, such as scanning speed, accumulations, and nitrogen flow rate, significantly impact the quality and reliability of the acquired CD spectra. Data processing is a critical step in obtaining accurate and interpretable CD spectra. Baseline correction, smoothing, and conversion to mean residue ellipticity are essential for reliable secondary structure analysis.

摘要

二级结构是指多肽主链通过氢键形成的高度规则的局部子结构。二级结构的两种主要类型是α螺旋和β链(可形成β折叠)。开发一种强大的用于生物分子结构分析的圆二色性(CD)方法需要仔细考虑几个关键因素。溶剂选择在维持样品的天然构象或所需构象同时确保在相关波长区域的透明度方面起着至关重要的作用。对于研究处于天然状态的蛋白质,水性缓冲液通常是首选。优化样品浓度和光程长度对于实现最佳吸光度范围并最大化信噪比至关重要。远紫外CD测量的典型浓度范围为0.1至1mg/ml,较短的光程长度(1mm)允许使用较高浓度,而较长的光程长度(5mm)适用于稀溶液。仪器参数,如扫描速度、累加次数和氮气流量,会显著影响所采集CD光谱的质量和可靠性。数据处理是获得准确且可解释的CD光谱的关键步骤。基线校正、平滑处理以及转换为平均残基椭圆率对于可靠的二级结构分析至关重要。

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