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人血清白蛋白在拥挤的 Pluronic F127 水凝胶中的结构、活性和动力学。

Structure, Activity, and Dynamics of Human Serum Albumin in a Crowded Pluronic F127 Hydrogel.

机构信息

Department of Chemistry , Indian Institute of Science Education and Research Bhopal , Bhopal Bypass Road , Bhopal 462066 , Madhya Pradesh , India.

School of Chemical Sciences , Indian Association for the Cultivation of Science , Jadavpur, Kolkata 700032 , India.

出版信息

J Phys Chem B. 2019 Apr 25;123(16):3397-3408. doi: 10.1021/acs.jpcb.9b00219. Epub 2019 Apr 17.

DOI:10.1021/acs.jpcb.9b00219
PMID:30945876
Abstract

Structure, activity, and dynamics of a plasma protein, human serum albumin (HSA), inside a crowded environment of F127 gel are studied by circular dichroism (CD), fluorescence correlation spectroscopy (FCS), and picosecond time-resolved fluorescence spectroscopy. For this purpose, the protein is covalently labeled by a maleimide dye, 7-(diethylamino)-3-(4-maleimidylphenyl)-4-methyl-coumarin (CPM). The circular dichroism (CD) spectra suggest that the protein is more structured in the gel reflecting about the biological activities of the protein. FCS results demonstrate that compared to that in bulk water (buffer solution), translational diffusion is about 59 times slower inside the F127 gel. This indicates higher translational friction (viscosity) sensed by the probe (CPM). On the contrary, rotational relaxation (and hence, rotational friction) is more or less similar in F127 gel and in bulk water. FCS results further indicate that the time scales of conformational relaxation of the protein are substantially slow inside the crowded environment of F127 gel. The fast component of conformational relaxation is retarded by ∼55 times, and the slow component by ∼20 times. Fluorescence maximum of CPM bound to HSA show a ∼5 nm red shift, implying that the microenvironment of the probe, CPM, is more polar inside the gel. Solvation dynamics of CPM-labeled HSA inside the gel (⟨τ⟩ ∼ 300 ps) is faster compared to that for the protein in bulk water (⟨τ⟩ ∼ 600 ps).

摘要

利用圆二色性(CD)、荧光相关光谱(FCS)和皮秒时间分辨荧光光谱研究了在 F127 凝胶拥挤环境中,血浆蛋白人血清白蛋白(HSA)的结构、活性和动力学。为此,通过马来酰亚胺染料 7-(二乙基氨基)-3-(4-马来酰亚胺基苯基)-4-甲基香豆素(CPM)对蛋白质进行共价标记。圆二色性(CD)谱表明,蛋白质在凝胶中更具结构,反映了蛋白质的生物学活性。FCS 结果表明,与在体相水中(缓冲溶液)相比,探针(CPM)在 F127 凝胶中的平动扩散大约慢 59 倍。这表明探针感受到更高的平动摩擦(粘度)。相反,在 F127 凝胶和体相水中,旋转弛豫(因此,旋转摩擦)或多或少相似。FCS 结果进一步表明,在 F127 凝胶拥挤环境中,蛋白质构象弛豫的时间尺度大大减慢。构象弛豫的快组分被延迟约 55 倍,慢组分被延迟约 20 倍。CPM 与 HSA 结合的荧光最大峰值发生约 5nm 的红移,这意味着探针 CPM 的微环境在凝胶内部更具极性。CPM 标记的 HSA 在内凝胶中的溶剂化动力学(⟨τ⟩∼300ps)比在体相水中的蛋白质更快(⟨τ⟩∼600ps)。

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