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首页> 外文期刊>Analytical methods >Coomassie Brilliant Blue-binding: a simple and effective method for the determination of water-insoluble protein surface hydrophobicity
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Coomassie Brilliant Blue-binding: a simple and effective method for the determination of water-insoluble protein surface hydrophobicity

机译:考马斯亮蓝结合:测定水不溶性蛋白质表面疏水性的简单有效方法

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摘要

A simple and convenient method for water-insoluble protein surface hydrophobicity determination was developed and validated. The method is based on the non-covalent binding of Coomassie Brilliant Blue G-250 (CBBG) to aromatic and basic amino acid residues on the surface of proteins, generating insoluble proteina€“CBBG complexes that could be precipitated by centrifugation and cause a reduction in the absorbance at 585 nm in the supernatant. The amount of protein-bound CBBG is applied as an indicator of protein surface hydrophobicity. Thermally treated, water-insoluble myofibrillar proteins (MPs) were chosen to validate the proposed method. The amount of protein-bound CBBG increased in thermally treated protein samples and the results were compared with the surface hydrophobicity (S0) calculated by the commonly accepted fluorescence method using a 1-anilino-8-naphthalenesulfonate (ANS) probe and intrinsic tryptophan fluorescence. Results from the CBBG-binding method linearly correlated with the S0 of the ANS fluorescence method (R = 0.95), the maximum emission wavelength of protein intrinsic fluorescence (R = 0.96) and the intrinsic fluorescence intensity at 337 nm (R = a?’0.73), strongly suggesting the reliability of the proposed CBBG-binding method.
机译:开发并验证了一种简便的测定水不溶性蛋白质表面疏水性的方法。该方法基于考马斯亮蓝G-250(CBBG)与蛋白质表面上的芳香族和碱性氨基酸残基的非共价结合,生成不溶性蛋白质-CBBG复合物,可通过离心作用沉淀并引起还原。上清液在585 nm处的吸光度。结合蛋白的CBBG的量被用作蛋白表面疏水性的指标。选择经过热处理的水不溶性肌原纤维蛋白(MPs)来验证所提出的方法。热处理后的蛋白质样品中结合蛋白质的CBBG的数量增加,并将结果与​​使用1-苯胺基-8-萘磺酸盐(ANS)探针和固有色氨酸荧光通过常用的荧光方法计算的表面疏水性(S0)进行比较。 CBBG结合法的结果与ANS荧光法的S0(R = 0.95),蛋白质固有荧光的最大发射波长(R = 0.96)和337 nm(R = a?' 0.73),强烈暗示了所提出的CBBG结合方法的可靠性。

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