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Quality control of protein crystal suspensions using microflow imaging and flow cytometry

机译:使用微流成像和流式细胞仪对蛋白质晶体悬浮液进行质量控制

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摘要

Protein crystallization is an attractive method for protein processing and formulation. However, minor changes in the crystallization setup can lead to changes in the crystal structure or the formation of amorphous protein aggregates, which affect the product quality. Only few analytical tools for qualitative and quantitative differentiation between protein crystals and amorphous protein exist. Electron microscopy requires expensive instrumentation, demanding sample preparation, and challenging image analysis. Therefore, there is a need to establish other analytical techniques. It was the aim of this study to investigate the capability of light obscuration (LO), microflow imaging (MFI), and flow cytometry (FC) in differentiating the amorphous and crystalline states of insulin as a relevant model. Qualitative discrimination of the two populations based on the particle size was possible using LO. Quantitative determination of amorphous protein and crystals by MFI was challenging due to overlapping size distributions. This problem was overcome by particle analysis based on the mean light intensity. Additionally, FC was applied as a new method for the determination of the quality and quantity of amorphous protein by differences in the light scattering. Our results show the potential of MFI and FC for rapid high throughput screening of crystallization conditions and product quality.
机译:蛋白质结晶是蛋白质加工和配制的一种有吸引力的方法。但是,结晶设置中的细微变化会导致晶体结构发生变化或形成无定形蛋白质聚集体,从而影响产品质量。只有很少的分析工具可用于定性和定量区分蛋白质晶体和无定形蛋白质。电子显微镜需要昂贵的仪器,要求样品准备和具有挑战性的图像分析。因此,需要建立其他分析技术。这项研究的目的是研究光遮蔽(LO),微流成像(MFI)和流式细胞仪(FC)在区分胰岛素的无定形和结晶状态方面的能力。使用LO可以根据粒径对两个种群进行定性鉴别。由于重叠的尺寸分布,通过MFI定量测定无定形蛋白质和晶体具有挑战性。通过基于平均光强度的粒子分析克服了这个问题。另外,FC被用作一种通过光散射差异确定非晶蛋白质的质量和数量的新方法。我们的结果显示了MFI和FC在快速高通量筛选结晶条件和产品质量方面的潜力。

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