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水溶液和水凝胶中明胶聚合物的荧光原位标记。

Fluorogenic in-situ Labelling of Gelatin Polymer in Aqueous Solution and Hydrogel.

机构信息

Shenzhen Research Institute of Hunan University, Nanshan District, Shenzhen, 518000, China.

State Key Laboratory of Chemo/Biosensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan University, Changsha, 410082, China.

出版信息

Chemistry. 2024 Sep 16;30(52):e202401561. doi: 10.1002/chem.202401561. Epub 2024 Aug 30.

DOI:10.1002/chem.202401561
PMID:38847762
Abstract

Gelatin polymers made from partially degraded collagen are important biomaterials, but their in-situ analysis suffers from uncontrollable covalent labelling and poor spatial-temporal imaging resolution. Herein, three tetrazolate-tagged tetraphenylethylene fluorophores (TPE-TAs) are introduced for practical fluorogenic labelling of gelatin in aqueous phase and hydrogels. These probes with aggregation-induced emission characteristics offer negligible background and elicit turn-on fluorescence by simply mixing with the gelatin in aqueous phase, giving a detection limit of 0.15 mg/L over a linear dynamic range up to 100 mg/L. This method does not work for collagens and causes minimal interference with gelatin properties. Mechanistic studies reveal a key role for multivalent electrostatic interactions between the abundant basic residues in gelatin (e. g., lysine, hydroxylysine, arginine) and anionic tetrazolate moieties of the lipophilic fluorophore synergistically in spatially rigid macromolecular encapsulation to achieve fluorogenic labelling. The AIE strategy by forming non-covalent fluorophore-gelatin complexes was developed for novel hydrogels that exhibited reversible fluorescence in response to dynamic microstructural changes in the hydrogel scaffold upon salting-in/out treatments, and enabled high spatial-temporal imaging of the fiber network in lyophilized samples. This work may open up avenues for in-situ imaging analysis and evaluation of gelatin-based biomaterials during processes such as in vivo degradation and mineralization.

摘要

部分降解胶原制成的明胶聚合物是重要的生物材料,但它们的原位分析受到不可控的共价标记和较差的时空成像分辨率的限制。在此,引入了三种四唑标记的四苯乙烯荧光团(TPE-TAs),用于在水相和水凝胶中对明胶进行实际的荧光标记。这些具有聚集诱导发射特性的探针背景信号可忽略不计,只需与水相中的明胶简单混合,即可产生开-关荧光,检测限低至 0.15mg/L,线性动态范围高达 100mg/L。该方法不适用于胶原蛋白,并对明胶性质的干扰最小。机理研究表明,明胶中丰富的碱性残基(如赖氨酸、羟赖氨酸、精氨酸)与疏水性荧光团的阴离子四唑部分之间的多价静电相互作用在空间刚性大分子包封中协同作用,对实现荧光标记起着关键作用。通过形成非共价的荧光团-明胶配合物的 AIE 策略,开发了新型水凝胶,该水凝胶在盐溶/盐析处理时,对水凝胶支架的动态微观结构变化表现出可逆荧光,并能够对冻干样品中的纤维网络进行高时空成像。这项工作可能为体内降解和矿化等过程中明胶基生物材料的原位成像分析和评估开辟新途径。

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