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利用细胞外中链长度聚羟基烷酸酯解聚酶将蛋白质靶向结合到人工聚[(3-羟基辛酸酯)-共-(3-羟基己酸酯)]颗粒上。

Use of extracellular medium chain length polyhydroxyalkanoate depolymerase for targeted binding of proteins to artificial poly[(3-hydroxyoctanoate)-co-(3-hydroxyhexanoate)] granules.

机构信息

Laboratory of Biomaterials, Swiss Federal Laboratories for Materials Testing and Research (EMPA), CH-9014 St. Gallen, Switzerland.

出版信息

Biomacromolecules. 2009 Jul 13;10(7):1854-64. doi: 10.1021/bm9002859. Epub 2009 May 21.

DOI:10.1021/bm9002859
PMID:19459673
Abstract

Polyhydroxyalkanoates (PHA), which are produced by many microorganisms, are promising polymers for biomedical applications due to their biodegradability and biocompatibility. In this study, we evaluated the suitability of medium chain length (mcl) PHA as surface materials for immobilizing proteins. Self-stabilized, artificial mcl-PHA beads with a size of 200-300 nm were fabricated. Five of six tested proteins adsorbed nonspecifically to mcl-PHA beads in amounts of 0.4-1.8 mg m(-2) bead surface area. The binding capacity was comparable to similar-sized polystyrene particles commonly used for antibody immobilization in clinical diagnostics. A targeted immobilization of fusion proteins was achieved by using inactive extracellular PHA depolymerase (ePHA(mcl)) from Pseudomonas fluorescens as the capture ligand. The N-terminal part of ePhaZ(MCL) preceding the catalytic domain was identified to comprise the substrate binding domain and was sufficient for mediating the binding of fusion proteins to mcl-PHA. We suggest mcl-PHA to be prime candidates for both nonspecific and targeted immobilization of proteins in applications such as drug delivery, protein microarrays, and protein purification.

摘要

聚羟基烷酸酯(PHA)由许多微生物产生,由于其可生物降解性和生物相容性,是用于生物医学应用的有前途的聚合物。在这项研究中,我们评估了中链长度(mcl)PHA 作为固定蛋白质的表面材料的适用性。制备了尺寸为 200-300nm 的自稳定的人工 mcl-PHA 珠。六种测试蛋白中有五种以 0.4-1.8mg m(-2)珠表面积的量非特异性吸附到 mcl-PHA 珠上。结合能力与临床诊断中常用的用于抗体固定的类似大小的聚苯乙烯颗粒相当。通过使用假单胞菌荧光素(Pseudomonas fluorescens)的无活性胞外 PHA 解聚酶(ePHA(mcl))作为捕获配体,实现了融合蛋白的靶向固定。鉴定出位于催化结构域之前的外 PHaZ(MCL)的 N 端部分包含底物结合结构域,足以介导融合蛋白与 mcl-PHA 的结合。我们建议 mcl-PHA 是药物输送、蛋白质微阵列和蛋白质纯化等应用中固定蛋白质的非特异性和靶向固定的主要候选物。

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