Thiele Thomas, Steil Leif, Völker Uwe, Greinacher Andreas
Institute of Immunology and Transfusion Medicine, Ernst-Moritz-Arndt University, Greifswald, Germany.
BioDrugs. 2007;21(3):179-93. doi: 10.2165/00063030-200721030-00005.
Blood-based therapeutics are cellular or plasma components derived from human blood. Their production requires appropriate selection and treatment of the donor and processing of cells or plasma proteins. In contrast to clearly defined, chemically synthesized drugs, blood-derived therapeutics are highly complex mixtures of plasma proteins or even more complex cells. Pathogen transmission by the product as well as changes in the integrity of blood constituents resulting in loss of function or immune modulation are currently important issues in transfusion medicine. Protein modifications can occur during various steps of the production process, such as acquisition, enrichment of separate components (e.g. coagulation factors, cell populations), virus inactivation, conservation, and storage. Contemporary proteomic strategies allow a comprehensive assessment of protein modifications with high coverage, offer capabilities for qualitative and even quantitative analysis, and for high-throughput protein identification. Traditionally, proteomics approaches predominantly relied on two-dimensional gel electrophoresis (2-DE). Even if 2-DE is still state of the art, it has inherent limitations that are mainly based on the physicochemical properties of the proteins analyzed; for example, proteins with extremes in molecular mass and hydrophobicity (most membrane proteins) are difficult to assess by 2-DE. These limitations have fostered the development of mass spectrometry centered on non-gel-based separation approaches, which have proven to be highly successful and are thus complementing and even partially replacing 2-DE-based approaches. Although blood constituents have been extensively analyzed by proteomics, this technology has not been widely applied to assess or even improve blood-derived therapeutics, or to monitor the production processes. As proteomic technologies have the capacity to provide comprehensive information about changes occurring during processing and storage of blood products, proteomics can potentially guide improvement of pathogen inactivation procedures and engineering of stem cells, and may also allow a better understanding of factors influencing the immunogenicity of blood-derived therapeutics. An important development in proteomics is the reduction of inter-assay variability. This now allows the screening of samples taken from the same product over time or before and after processing. Optimized preparation procedures and storage conditions will reduce the risk of protein alterations, which in turn may contribute to better recovery, reduced exposure to allogeneic proteins, and increased transfusion safety.
血液制品是源自人血的细胞或血浆成分。其生产需要对供体进行适当的选择和处理,并对细胞或血浆蛋白进行加工。与明确界定的化学合成药物不同,血液制品是血浆蛋白的高度复杂混合物,甚至是更复杂的细胞。目前,输血医学中的重要问题包括产品导致的病原体传播以及血液成分完整性的改变,进而导致功能丧失或免疫调节。蛋白质修饰可能发生在生产过程的各个步骤中,如采集、分离成分(如凝血因子、细胞群体)的富集、病毒灭活、保存和储存。当代蛋白质组学策略能够对蛋白质修饰进行全面评估,覆盖范围广,具备定性甚至定量分析以及高通量蛋白质鉴定的能力。传统上,蛋白质组学方法主要依赖二维凝胶电泳(2-DE)。即使2-DE仍然是最先进的技术,但它存在一些固有局限性,主要基于所分析蛋白质的物理化学性质;例如,分子量和疏水性极端的蛋白质(大多数膜蛋白)难以通过2-DE进行评估。这些局限性推动了以非凝胶分离方法为中心的质谱技术的发展,事实证明该技术非常成功,因此正在补充甚至部分取代基于2-DE的方法。尽管蛋白质组学已广泛分析了血液成分,但该技术尚未广泛应用于评估甚至改进血液制品,或监测生产过程。由于蛋白质组学技术有能力提供关于血液制品加工和储存过程中发生变化的全面信息,蛋白质组学有可能指导病原体灭活程序的改进和干细胞工程,还可能有助于更好地理解影响血液制品免疫原性的因素。蛋白质组学的一个重要发展是减少分析间的变异性。现在这使得能够对同一产品在不同时间或加工前后采集的样本进行筛选。优化的制备程序和储存条件将降低蛋白质改变的风险,这反过来可能有助于提高回收率、减少异体蛋白暴露并提高输血安全性。
