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脂质体包裹血红蛋白中内毒素准确测量的比较研究。

A comparative study of the accurate measurement of endotoxin in liposome-encapsulated hemoglobin.

作者信息

Cliff R O, Kwasiborski V, Rudolph A S

机构信息

Center for BioMolecular Science and Engineering, Naval Research Laboratory, Washington, DC 20375-5348, USA.

出版信息

Artif Cells Blood Substit Immobil Biotechnol. 1995;23(3):331-6. doi: 10.3109/10731199509117949.

Abstract

We have examined three different methods of endotoxin determination utilizing the Limulus Amebocyte Lysate (LAL) assay to accurately determine endotoxin levels in Liposome Encapsulated Hemoglobin (LEH), 1) the gel-clot method, 2) chromogenic spectroscopic-based LAL, and 3) the turbidimetric method which determines endotoxin levels in solutions based on the time needed to reach a specific degree of turbidity. Both the chromogenic and turbidimetric methods require significant dilution of the LEH preparation before accurate measurement can be made. We have tested the levels of endotoxin in LEH solutions using these methods and measured LEH, liposome, and hemoglobin samples spiked with known amounts of endotoxin. A comparison of the three methods shows that the absolute value of endotoxin measured in LEH by the three methods can vary significantly. However, within any one assay the spiked amount of endotoxin in the sample can be accurately measured. The accuracy of these methods may also be complicated by the binding of endotoxin to LEH. This was evident by mixing free endotoxin with LEH followed by centrifugation to separate the LEH. Biological activity of endotoxin bound to LEH was measured by exposure to RAW264.7 followed by the expression of tumor necrosis factor.

摘要

我们使用鲎试剂(LAL)测定法研究了三种不同的内毒素测定方法,以准确测定脂质体包裹血红蛋白(LEH)中的内毒素水平,1)凝胶凝块法,2)基于显色光谱的鲎试剂法,以及3)比浊法,该方法根据达到特定浊度所需的时间来测定溶液中的内毒素水平。在进行准确测量之前,显色法和比浊法都需要对LEH制剂进行大量稀释。我们使用这些方法测试了LEH溶液中的内毒素水平,并测量了添加了已知量内毒素的LEH、脂质体和血红蛋白样品。三种方法的比较表明,三种方法在LEH中测得的内毒素绝对值可能有显著差异。然而,在任何一种测定中,样品中添加的内毒素量都可以准确测量。内毒素与LEH的结合也可能使这些方法的准确性变得复杂。将游离内毒素与LEH混合,然后离心分离LEH,这一点很明显。通过将与LEH结合的内毒素暴露于RAW264.7细胞,然后检测肿瘤坏死因子的表达来测量其生物活性。

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