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酸性成纤维细胞生长因子的制剂设计

Formulation design of acidic fibroblast growth factor.

作者信息

Tsai P K, Volkin D B, Dabora J M, Thompson K C, Bruner M W, Gress J O, Matuszewska B, Keogan M, Bondi J V, Middaugh C R

机构信息

Department of Pharmaceutical Research, Merck Research Laboratory, West Point, Pennsylvania 19486.

出版信息

Pharm Res. 1993 May;10(5):649-59. doi: 10.1023/a:1018939228201.

DOI:10.1023/a:1018939228201
PMID:7686672
Abstract

The design of an aqueous formulation for acidic fibroblast growth factor (aFGF) requires an understanding of the type of compounds that can either directly or indirectly stabilize the protein. To this end, spectrophotometric turbidity measurements were initially employed to screen the ability of polyanionic ligands, less specific compounds, and variations in solution conditions (temperature and pH) to stabilize aFGF against heat-induced aggregation. It was found that in addition to the well-known protection of aFGF by heparin, a surprisingly wide variety of polyanions (including small sulfated and phosphorylated compounds) also stabilizes aFGF. These polyanionic ligands are capable of raising the temperature at which the protein unfolds by 15-30 degrees C. Many commonly used excipients were also observed to stabilize aFGF in both the presence and the absence of heparin. High concentrations of some of these less specific agents are also able to increase the temperature of aFGF thermal unfolding by as much as 6-12 degrees C as shown by circular dichroism and differential scanning calorimetry. Other compounds were found which protect the chemically labile cysteine residues of aFGF from oxidation. Aqueous formulations of aFGF were thus designed to contain both a polyanionic ligand that enhances structural integrity by binding to the protein and chelating agents (e.g., EDTA) to prevent metal ion-catalyzed oxidation of cysteine residues. While room-temperature storage (30 degrees C) leads to rapid inactivation of aFGF in physiological buffer alone, several of these aFGF formulations are stable in vitro for at least 3 months at 30 degrees C. Three aFGF topical formulations were examined in an impaired diabetic mouse model and were found to be equally capable of accelerating wound healing.

摘要

设计酸性成纤维细胞生长因子(aFGF)的水性制剂需要了解能够直接或间接稳定该蛋白质的化合物类型。为此,最初采用分光光度法浊度测量来筛选聚阴离子配体、特异性较低的化合物以及溶液条件(温度和pH)的变化对aFGF抗热诱导聚集的稳定能力。结果发现,除了肝素对aFGF的众所周知的保护作用外,令人惊讶的是,多种聚阴离子(包括小的硫酸化和磷酸化化合物)也能稳定aFGF。这些聚阴离子配体能够使蛋白质展开的温度提高15 - 30摄氏度。还观察到许多常用辅料在有肝素和无肝素的情况下都能稳定aFGF。圆二色光谱和差示扫描量热法表明,其中一些特异性较低的试剂在高浓度时也能使aFGF热展开温度提高多达6 - 12摄氏度。还发现了其他化合物可以保护aFGF化学性质不稳定的半胱氨酸残基不被氧化。因此,aFGF的水性制剂设计为既含有通过与蛋白质结合增强结构完整性的聚阴离子配体,又含有螯合剂(如EDTA)以防止金属离子催化的半胱氨酸残基氧化。虽然仅在生理缓冲液中于室温(30摄氏度)储存会导致aFGF迅速失活,但这些aFGF制剂中的几种在30摄氏度下体外至少稳定3个月。在糖尿病受损小鼠模型中对三种aFGF局部制剂进行了检查,发现它们同样能够加速伤口愈合。

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Formulation design of acidic fibroblast growth factor.酸性成纤维细胞生长因子的制剂设计
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Nature of the interaction of heparin with acidic fibroblast growth factor.肝素与酸性成纤维细胞生长因子的相互作用性质
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Physical stabilization of acidic fibroblast growth factor by polyanions.多聚阴离子对酸性成纤维细胞生长因子的物理稳定作用。
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Acidic fibroblast growth factor: evaluation of topical formulations in a diabetic mouse wound healing model.酸性成纤维细胞生长因子:在糖尿病小鼠伤口愈合模型中对局部制剂的评估
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