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通过庚烷 - 水分配法测定的白蛋白 - 脂肪酸结合常数的校准。

Calibration of albumin-fatty acid binding constants measured by heptane-water partition.

作者信息

Burczynski F J, Pond S M, Davis C K, Johnson L P, Weisiger R A

机构信息

Department of Medicine, University of California, San Francisco 94143-0538.

出版信息

Am J Physiol. 1993 Sep;265(3 Pt 1):G555-63. doi: 10.1152/ajpgi.1993.265.3.G555.

DOI:10.1152/ajpgi.1993.265.3.G555
PMID:8214076
Abstract

Most measurements of binding affinity of albumin for long-chain fatty acids are based on heptane-water partition. In this method, equilibrium partition of fatty acid between heptane and an albumin-containing buffer is calibrated using the partition ratio between heptane and buffer in the absence of protein. In the current study, we used a variety of techniques to examine potential problems with this approach. Hydrophobic impurities in commercial [3H]palmitate preparations were incompletely removed by standard purification techniques. These impurities contributed from 5% of the total radioactivity in the heptane phase at low albumin concentrations (5 microM) to 62% at higher albumin concentrations (500 microM), thus confounding determination of binding affinity. These were identified by gas chromatography/mass spectroscopy as radio-labeled glycerol monopalmitate and monostearate. When albumin was not present, the partition ratio was similar to values reported by others. However, our results varied by a factor of four (265-1,119) depending on how the solutions were prepared. Although a true equilibrium partition must not depend on starting conditions, the partition ratio after 24-72 h was > 2x as large when tracer [3H]palmitate was added to the heptane phase than when it was added to the aqueous phase. Results also depended on the relative volumes of heptane and buffer used, approaching a maximum of 1,445 +/- 112 for very low heptane/buffer volume ratios. Much of this variability was due to hydrophilic impurities in [3H]palmitate, which ranged from 0.2 to 1.2% in commercial lots down to 0.1-0.5% after alkaline ethanol extraction and < 0.05% after thin-layer chromatography (TLC).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

大多数关于白蛋白与长链脂肪酸结合亲和力的测量都是基于庚烷 - 水分配法。在该方法中,脂肪酸在庚烷和含白蛋白缓冲液之间的平衡分配是通过在无蛋白质情况下庚烷与缓冲液之间的分配比来校准的。在本研究中,我们使用了多种技术来检查这种方法存在的潜在问题。市售[³H]棕榈酸制剂中的疏水杂质不能通过标准纯化技术完全去除。这些杂质在低白蛋白浓度(5微摩尔)时占庚烷相总放射性的5%,在高白蛋白浓度(500微摩尔)时占62%,从而混淆了结合亲和力的测定。通过气相色谱/质谱法鉴定这些杂质为放射性标记的甘油单棕榈酸酯和单硬脂酸酯。当不存在白蛋白时,分配比与其他人报道的值相似。然而,我们的结果因溶液制备方式的不同而相差四倍(265 - 1119)。尽管真正的平衡分配不应依赖于起始条件,但当示踪剂[³H]棕榈酸添加到庚烷相时,24 - 72小时后的分配比比添加到水相时大2倍以上。结果还取决于所用庚烷和缓冲液的相对体积,对于非常低的庚烷/缓冲液体积比,接近最大值1445±112。这种变异性很大程度上是由于[³H]棕榈酸中的亲水杂质,商业批次中的亲水杂质含量在0.2%至1.2%之间,经碱性乙醇萃取后降至0.1% - 0.5%,经薄层色谱(TLC)后<0.05%。(摘要截断于250字)

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