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采用生物素标记的透明质酸结合蛋白的夹心 ELISA 样测定和膜印迹法检测透明质酸的分子质量依赖性。

Molecular mass dependence of hyaluronan detection by sandwich ELISA-like assay and membrane blotting using biotinylated hyaluronan binding protein.

机构信息

Department of Chemical and Biomolecular Engineering, Polytechnic Institute of New York University, 6 Metrotech Center, Brooklyn, NY 11201, USA.

出版信息

Glycobiology. 2013 Nov;23(11):1270-80. doi: 10.1093/glycob/cwt064. Epub 2013 Aug 19.

DOI:10.1093/glycob/cwt064
PMID:23964097
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3796376/
Abstract

Hyaluronan (HA) is widely detected in biological samples and its concentration is most commonly determined by the use of a labeled specific HA binding protein (aggrecan G1-IGD-G2, HABP), employing membrane blotting and sandwich enzyme-linked immunosorbent assay (ELISA)-like methods. However, the detected signal intensity or the quantified value obtained by using these surface-based methods is related to the molecular mass (M) of HA, especially for HA in the low M range below ~150 kDa. At the same mass or mass concentration, higher M HA gives a higher signal than lower M HA. We have experimentally determined the quantitative relationship between the M of HA (in the range 20-150 kDa) and the relative signal intensity in comparison with a standard HA, in a sandwich ELISA-like assay. An M-dependent signal correction factor (SCF) was calculated and used to correct the signal intensity, so that the corrected concentration value would more accurately reflect the true HA concentration in solution. The SCF for polydisperse low M HA was also calculated and compared with experimental results. When the molecular mass distribution of an HA sample is determined by a method such as gel electrophoresis, then its appropriately averaged SCF can be calculated and used to correct the signal in sandwich ELISA to obtain a more accurate concentration estimation. The correction method works for HA with M between ~150 and 20 kDa, but lower M HA is too poorly detected for useful analysis. The physical basis of the M-dependent detection is proposed to be the increase in detector-accessible fraction of each surface-bound molecule as M increases.

摘要

透明质酸(HA)广泛存在于生物样本中,其浓度通常通过使用标记的特定 HA 结合蛋白(聚集蛋白 G1-IGD-G2,HABP)来确定,采用膜印迹和夹心酶联免疫吸附测定(ELISA)样方法。然而,使用这些基于表面的方法检测到的信号强度或定量值与 HA 的分子量(M)有关,特别是对于低于150 kDa 的低 M 范围的 HA。在相同的质量或质量浓度下,较高 M 的 HA 比较低 M 的 HA 产生更高的信号。我们在夹心 ELISA 样测定中实验确定了 HA 的 M(20-150 kDa 范围内)与相对信号强度之间的定量关系,与标准 HA 进行比较。计算了与 M 相关的信号校正因子(SCF),并用于校正信号强度,以便校正后的浓度值更准确地反映溶液中真实的 HA 浓度。还计算了多分散低 M HA 的 SCF,并与实验结果进行了比较。当通过诸如凝胶电泳的方法确定 HA 样品的分子量分布时,可以计算其适当平均的 SCF 并用于校正夹心 ELISA 中的信号,以获得更准确的浓度估计。该校正方法适用于 M 在150 和 20 kDa 之间的 HA,但对于有用的分析,较低 M 的 HA 检测效果较差。M 依赖性检测的物理基础被提出为随着 M 的增加,每个表面结合分子的可检测部分增加。

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