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采用适当的理化和功能策略组合,在输液袋中制备的 ziv-aflibercept 临床溶液的时间稳定性研究。

Stability study over time of clinical solutions of ziv-aflibercept prepared in infusion bags using a proper combination of physicochemical and functional strategies.

机构信息

Department of Analytical Chemistry, Sciences Faculty, Instituto de Investigación Biosanitaria (ibs.Granada), University of Granada, E-18071, Granada, Spain.

Department of Clinical Pharmacy, Instituto de Investigación Biosanitaria (ibs.Granada), San Cecilio University Hospital, 18016, Granada, Spain.

出版信息

J Pharm Biomed Anal. 2021 Sep 5;203:114209. doi: 10.1016/j.jpba.2021.114209. Epub 2021 Jun 16.

Abstract

A range of biopharmaceutical products are used to target Vascular Endothelial Growth Factor (VEGF), including Eylea® (aflibercept, AFL) and Zaltrap® (ziv-aflibercept, ziv-AFL). The first is indicated for ophthalmological diseases such as neovascular (wet) age-related macular degeneration, while the second is used in the treatment of metastatic colorectal cancer. The stability of AFL in prefilled syringes has been widely studied; however, no research has yet been done on the stability of ziv-AFL in polyolefin infusion bags. Therefore, the purpose of the present research is to evaluate the stability of ziv-AFL (Zaltrap®) clinical solutions prepared under aseptic conditions in polyolefin infusion bags at two different concentrations, i.e. 4.0 and 0.6 mg/mL, and stored refrigerated in darkness at 2-8 °C for 14 days. With that aim, the ziv-AFL clinical solutions were assessed by analysing changes in its physicochemical and functional properties. The distribution of the particulates was studied over a range of 0.001-10 μm by Dynamic Light Scattering (DLS); oligomers were analysed by Size-Exclusion High-Performance Chromatography with Diode Array Detection (SE/HLPC-DAD); the secondary structure of the protein was studied by far UV Circular Dichroism (CD) and the tertiary structure by Intrinsic Tryptophan Fluorescence (IT-F) and Intrinsic Protein Fluorescence (IP-F); charge variants were assessed by Strong Cation Exchange Ultra-High-Performance Chromatography with UV detection (SCX/UHPLC-UV); functionality was evaluated by ELISA by measuring the biological activity as manifested in the extension of the immunological reaction of the ziv-AFL with its antigen (VEGF). Neither aggregation nor oligomerization were detected by the techniques mentioned above. Secondary and tertiary structures remained unchanged over the 14-day period, as did charge variants. The functionality observed initially was maintained along time. Therefore, it could be proposed that the ziv-AFL clinical solutions studied showed great physicochemical and functional stability over a period of two weeks, regardless of the concentration, i.e. 4 or 0.6 mg/mL.

摘要

一系列的生物制药产品被用于靶向血管内皮生长因子(VEGF),包括艾力雅(阿柏西普,AFL)和赞可达(泽维仑赛,ziv-AFL)。前者用于治疗眼科疾病,如新生血管性(湿性)年龄相关性黄斑变性,而后者用于转移性结直肠癌的治疗。AFL 在预装注射器中的稳定性已经得到了广泛的研究;然而,目前还没有研究泽维仑赛(Zaltrap®)在聚烯烃输液袋中的稳定性。因此,本研究的目的是评估在无菌条件下制备的两种不同浓度(4.0 和 0.6mg/ml)的泽维仑赛(Zaltrap®)临床溶液在聚烯烃输液袋中的稳定性,这些溶液在 2-8°C 的黑暗环境下冷藏保存 14 天。为此,通过分析其物理化学和功能特性的变化来评估 ziv-AFL 临床溶液。通过动态光散射(DLS)研究了粒径分布在 0.001-10μm 范围内的情况;通过尺寸排阻高效液相色谱与二极管阵列检测(SE/HLPC-DAD)分析了低聚物;通过远紫外圆二色性(CD)研究了蛋白质的二级结构,通过内源色氨酸荧光(IT-F)和内源蛋白荧光(IP-F)研究了三级结构;通过强阳离子交换超高效液相色谱与紫外检测(SCX/UHPLC-UV)评估了电荷变异体;通过 ELISA 评估了功能,通过测量 ziv-AFL 与抗原(VEGF)的免疫反应的延伸来评估其生物学活性。上述技术均未检测到聚集或低聚物形成。二级和三级结构在 14 天内保持不变,电荷变异体也是如此。最初观察到的功能随着时间的推移而保持。因此,可以提出,在所研究的两周时间内,无论浓度为 4 或 0.6mg/ml,研究用的 ziv-AFL 临床溶液都表现出很好的物理化学和功能稳定性。

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