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生理体液和组织中胰岛素样生长因子-II的测定。I. 一种改进的人及大鼠体液提取方法和放射免疫分析法。

Measurement of insulin-like growth factor-II in physiological fluids and tissues. I. An improved extraction procedure and radioimmunoassay for human and rat fluids.

作者信息

Bowsher R R, Lee W H, Apathy J M, O'Brien P J, Ferguson A L, Henry D P

机构信息

Lilly Laboratory for Clinical Research, Eli Lilly Co., Indianapolis, Indiana.

出版信息

Endocrinology. 1991 Feb;128(2):805-14. doi: 10.1210/endo-128-2-805.

DOI:10.1210/endo-128-2-805
PMID:1989863
Abstract

The measurement of serum insulin-like growth factors (IGFs) in serum is complicated by the presence of high affinity IGF-binding proteins. The accurate measurement of IGFs by radioligand binding assays requires that the interference from binding proteins be eliminated. Acid-gel chromatography, the standard method for removing binding proteins, is laborious and time consuming. Alternative methods for extracting serum IGFs include the use of HCl-ethanol treatment and reverse phase minicolumns. However, these methods are unsuitable for use with serum for some species, such as rat and sheep, due to incomplete removal of binding proteins. We developed a fast protein liquid chromatography size-exclusion chromatographic method for characterizing the presence of IGF-binding proteins in physiological fluids and used this method to systematically investigate different combinations of acids and organic solvents as potential extraction methods for IGFs. We developed and validated an improved extraction procedure that uses formic acid, Tween-20, and acetone. The new extraction method was used in conjunction with purified biosynthetic human IGF-II and a commercially available anti-IGF-II monoclonal antibody in the development of an improved RIA for IGF-II. The new RIA is sensitive (5.0 pg/tube), specific (IGF-I cross-reactivity, less than 1%), and reproducible [interassay precision (coefficient of variation), less than 9.2%). We measured the serum concentrations of IGF-II in adults and found a significant difference between normal subjects and individuals with insulin-dependent diabetes mellitus.

摘要

血清中胰岛素样生长因子(IGFs)的测量因存在高亲和力的IGF结合蛋白而变得复杂。通过放射配体结合测定法准确测量IGFs需要消除结合蛋白的干扰。酸凝胶色谱法作为去除结合蛋白的标准方法,既费力又耗时。提取血清IGFs的替代方法包括使用盐酸 - 乙醇处理和反相微型柱。然而,由于结合蛋白去除不完全,这些方法不适用于某些物种(如大鼠和绵羊)的血清。我们开发了一种快速蛋白质液相色谱尺寸排阻色谱法,用于表征生理流体中IGF结合蛋白的存在,并使用该方法系统地研究酸和有机溶剂的不同组合作为IGFs的潜在提取方法。我们开发并验证了一种改进的提取程序,该程序使用甲酸、吐温 - 20和丙酮。在开发改进的IGF - II放射免疫分析方法时,将这种新的提取方法与纯化的生物合成人IGF - II和市售的抗IGF - II单克隆抗体结合使用。新的放射免疫分析方法灵敏(5.0 pg/管)、特异(IGF - I交叉反应性小于1%)且可重复[批间精密度(变异系数)小于9.2%]。我们测量了成年人血清中IGF - II的浓度,发现正常受试者与胰岛素依赖型糖尿病患者之间存在显著差异。

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