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载适配体的超顺磁性珠用于活化蛋白 C 的选择性捕获和温和释放。

Aptamer loaded superparamagnetic beads for selective capturing and gentle release of activated protein C.

机构信息

Institute of Experimental Hematology and Transfusion Medicine, University Hospital Bonn, 53127, Bonn, Germany.

Life and Medical Sciences Institute, University of Bonn, 53115, Bonn, Germany.

出版信息

Sci Rep. 2022 Apr 30;12(1):7091. doi: 10.1038/s41598-022-11198-5.

Abstract

Activated protein C (APC) is a serine protease with anticoagulant and cytoprotective activities which make it an attractive target for diagnostic and therapeutic applications. In this work, we present one-step activation of APC from a commercial source of protein C (PC, Ceprotin) followed by rapid and efficient purification using an APC-specific aptamer, HS02-52G, loaded on MyOne superparamagnetic beads. Due to the Ca-dependent binding of APC to HS02-52G, an efficient capturing of APC was applied in the presence of Ca ions, while a gentle release of captured APC was achieved in the elution buffer containing low EDTA concentration (5 mM). The captured and eluted APC showed more than 95% purity according to SDS-PAGE gel analysis and an enzyme-linked fluorescent assay (VIDAS Protein C). The purification yield of 45% was calculated when 4.2 µg APC was used, however this yield reduced to 21% if the starting amount of APC increased to 28.5 µg. Altogether, this method is recommended for rapid and efficient PC activation and APC purification. The purified APC can be used directly for downstream processes where high concentration of pure and active APC is needed.

摘要

活化蛋白 C(APC)是一种丝氨酸蛋白酶,具有抗凝和细胞保护活性,使其成为诊断和治疗应用的有吸引力的目标。在这项工作中,我们展示了一种从商业来源的蛋白 C(PC,Ceprotin)一步激活 APC 的方法,然后使用 APC 特异性适体 HS02-52G 进行快速有效的纯化,该适体加载在 MyOne 超顺磁珠上。由于 APC 与 HS02-52G 的 Ca 依赖性结合,在存在 Ca 离子的情况下,APC 的高效捕获得以实现,而在含有低 EDTA 浓度(5 mM)的洗脱缓冲液中,捕获的 APC 可温和释放。根据 SDS-PAGE 凝胶分析和酶联荧光测定(VIDAS 蛋白 C),捕获和洗脱的 APC 显示出超过 95%的纯度。当使用 4.2 µg APC 时,计算出 45%的纯化产率,但如果 APC 的起始量增加到 28.5 µg,则产率降低到 21%。总的来说,该方法推荐用于快速有效的 PC 激活和 APC 纯化。纯化的 APC 可直接用于需要高浓度纯 APC 的下游工艺。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b02/9056527/29c59dc35db5/41598_2022_11198_Fig1_HTML.jpg

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