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评价构建蛋白功能化的双离子囊泡的方法。

Evaluating methods to create protein functionalized catanionic vesicles.

机构信息

Chemistry Department, Saint Anselm College, Manchester, NH 03102, USA.

Department of Chemistry & Biochemistry, University of Maryland, College Park, MD 20742, USA.

出版信息

Soft Matter. 2023 Feb 15;19(7):1429-1439. doi: 10.1039/d2sm01205g.

Abstract

Catanionic surfactant vesicles (SVs) composed of sodium dodecylbenzenesulfonate (SDBS) and cetyltrimethylammonium tosylate (CTAT) have potential applications as targeted drug delivery systems, vaccine platforms, and diagnostic tools. To facilitate these applications, we evaluated various methods to attach proteins to the surface of SDBS/CTAT vesicles. Acid phosphatase from wheat germ was used as a model protein. Acid phosphatase was successfully conjugated to vesicles enriched with a Triton-X 100 derivative containing an unsaturated ester. Enzymatic activity of acid phosphatase attached to vesicles was assessed using an acid phosphatase assay. Results from the acid phosphatase assay indicated that 15 ± 3% of the attached protein remained functional but the presence of vesicles interferes with the assay. DLS and zeta potential results correlated with the protein functionalization studies. Acid phosphatase functionalized vesicles had an average diameter of 175 ± 85 nm and an average zeta potential of -61 ± 5 mV in PBS. As a control, vesicles enriched with Triton-X 100 were prepared and analyzed by DLS and zeta potential measurements. Triton X-100 enriched vesicles had an average diameter of 140 ± 67 nm and an average zeta potential of -49 ± 2 mV in PBS. Functionalizing the surface of SVs with proteins may be a key step in developing vesicle-based technologies. For drug delivery, antibodies could be used as targeting molecules; for vaccine formulation, functionalizing the surface with spike proteins may produce novel vaccine platforms.

摘要

由十二烷基苯磺酸钠(SDBS)和十六烷基三甲基溴化铵(CTAT)组成的混合离子型表面活性剂囊泡(SV)在作为靶向药物传递系统、疫苗平台和诊断工具方面具有潜在的应用。为了促进这些应用,我们评估了将蛋白质附着到 SDBS/CTAT 囊泡表面的各种方法。从小麦胚中提取的酸性磷酸酶被用作模型蛋白。成功地将酸性磷酸酶连接到富含含有不饱和酯的 Triton-X 100 衍生物的囊泡上。使用酸性磷酸酶测定法评估附着在囊泡上的酸性磷酸酶的酶活性。酸性磷酸酶测定结果表明,附着的蛋白质中有 15±3%保持功能,但囊泡的存在会干扰测定。DLS 和 zeta 电位结果与蛋白质功能化研究相关。在 PBS 中,酸性磷酸酶功能化囊泡的平均直径为 175±85nm,平均 zeta 电位为-61±5mV。作为对照,制备了富含 Triton-X 100 的囊泡,并通过 DLS 和 zeta 电位测量进行了分析。在 PBS 中,Triton X-100 富集囊泡的平均直径为 140±67nm,平均 zeta 电位为-49±2mV。用蛋白质对 SV 表面进行功能化可能是开发基于囊泡的技术的关键步骤。对于药物传递,可以将抗体用作靶向分子;对于疫苗制剂,用刺突蛋白对表面进行功能化可能会产生新型疫苗平台。

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