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人生物体液中胰岛素样生长因子结合蛋白-3的测定与特性分析:放射免疫测定法与配体印迹法之间的差异

Measurement and characterization of insulin-like growth factor binding protein-3 in human biological fluids: discrepancies between radioimmunoassay and ligand blotting.

作者信息

Gargosky S E, Pham H M, Wilson K F, Liu F, Giudice L C, Rosenfeld R G

机构信息

Department of Pediatrics, Stanford University School of Medicine, California 94305.

出版信息

Endocrinology. 1992 Dec;131(6):3051-60. doi: 10.1210/endo.131.6.1280211.

DOI:10.1210/endo.131.6.1280211
PMID:1280211
Abstract

The inability to detect insulin-like growth factor binding protein-3 (IGFBP-3) in some circumstances by Western ligand blot analysis has emphasized the need to characterize IGFBPs by both ligand binding and immunological techniques. In this study, we have: 1) characterized and quantified IGFBP-3 in nonpregnancy, pregnancy, and fetal cord serum, follicular, peritoneal, and amniotic fluid, seminal plasma, cerebrospinal fluid (CSF), and urine; 2) established a new IGFBP-3 RIA that detects both intact and fragments of IGFBP-3; 3) identified both intact and fragments of IGFBP-3 by Western immunoblot techniques; and 4) addressed the discordance between Western ligand blot analysis and RIA by assessing fluids for IGFBP proteolytic activity. All fluids examined, except pregnancy serum, CSF, and amniotic fluid, displayed a 44-34-kilodalton (kDa) IGFBP-3 doublet by Western ligand blot analysis. Western immunoblot analysis using specific IGFBP-3 antiserum showed a 44-34-kDa IGFBP-3 doublet and a 28-kDa fragment in nonpregnancy serum, fetal cord serum, follicular fluid, and peritoneal fluid. The immunoreactive 42-38-kDa doublet was faint in urine and seminal plasma. IGFBPs in CSF did not cross-react with IGFBP-3 antiserum. Pregnancy serum and amniotic fluid contained only the 28-kDa fragment when compared against equal volumes of nonpregnancy serum. With the development of an IGFBP-3 RIA, IGFBP-3 could be accurately measured; urine, CSF, and seminal plasma contained the lowest levels of IGFBP-3 at 27 +/- 3 ng/ml (mean +/- SEM), 110 +/- 26 ng/ml, and 209 +/- 56 ng/ml, respectively. In increasing concentration: fetal cord serum contained 753 +/- 101 ng/ml; peritoneal fluid, 1124 +/- 130 ng/ml; follicular fluid, 2356 +/- 211 ng/ml; nonpregnancy serum, 3556 +/- 508 ng/ml; pregnancy serum, 3718 +/- 842 ng/ml; and amniotic fluid, 5150 +/- 688 ng/ml. The measurable concentrations of IGFBP-3 in CSF and the high concentrations measured in pregnancy serum and amniotic fluid conflicted with Western blot analysis. Thus, fluids were assessed for IGFBP proteolytic activity by incubation with a source of IGFBP-3, either nonpregnancy serum or purified IGFBP-3. All fluids displayed some proteolytic activity with either assay. Fluids with little protease activity (nonpregnancy serum, follicular fluid, and urine) showed a close relationship between immunoassayable IGFBP-3 by RIA and IGFBP-3 band intensity by Western ligand blot. Fluids with high proteolytic activity (pregnancy serum, CSF, seminal plasma, peritoneal fluid, and amniotic fluid) gave discrepant IGFBP-3 values between RIA and Western ligand blot.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

在某些情况下,通过Western配体印迹分析无法检测到胰岛素样生长因子结合蛋白-3(IGFBP-3),这凸显了通过配体结合和免疫技术对IGFBPs进行表征的必要性。在本研究中,我们:1)对非妊娠、妊娠及胎儿脐带血清、卵泡液、腹腔液、羊水、精液、脑脊液(CSF)和尿液中的IGFBP-3进行了表征和定量;2)建立了一种新的IGFBP-3放射免疫分析方法(RIA),该方法可检测完整的和片段化的IGFBP-3;3)通过Western免疫印迹技术鉴定了完整的和片段化的IGFBP-3;4)通过评估液体中的IGFBP蛋白水解活性,解决了Western配体印迹分析与RIA之间的不一致问题。除妊娠血清、CSF和羊水外,所有检测的液体通过Western配体印迹分析均显示出44 - 34千道尔顿(kDa)的IGFBP-3双峰。使用特异性IGFBP-3抗血清的Western免疫印迹分析显示,非妊娠血清、胎儿脐带血清、卵泡液和腹腔液中存在44 - 34 kDa的IGFBP-3双峰和一个28 kDa的片段。免疫反应性42 - 38 kDa的双峰在尿液和精液中较淡。CSF中的IGFBPs与IGFBP-3抗血清无交叉反应。与等量非妊娠血清相比,妊娠血清和羊水中仅含有28 kDa的片段。随着IGFBP-3 RIA的发展,可准确测量IGFBP-3;尿液、CSF和精液中IGFBP-3的含量最低,分别为27±3 ng/ml(平均值±标准误)、110±26 ng/ml和209±56 ng/ml。浓度递增顺序为:胎儿脐带血清含有753±101 ng/ml;腹腔液,1124±130 ng/ml;卵泡液,2356±211 ng/ml;非妊娠血清,3556±508 ng/ml;妊娠血清,3718±842 ng/ml;羊水,5150±688 ng/ml。CSF中可测量的IGFBP-3浓度以及妊娠血清和羊水中测得的高浓度与Western印迹分析结果相矛盾。因此,通过与IGFBP-3来源(非妊娠血清或纯化的IGFBP-3)孵育来评估液体中的IGFBP蛋白水解活性。两种检测方法中所有液体均显示出一定的蛋白水解活性。蛋白酶活性低的液体(非妊娠血清、卵泡液和尿液)通过RIA检测的可免疫测定的IGFBP-3与通过Western配体印迹检测的IGFBP-3条带强度之间存在密切关系。蛋白酶活性高的液体(妊娠血清、CSF、精液、腹腔液和羊水)在RIA和Western配体印迹之间给出的IGFBP-3值存在差异。(摘要截断于400字)

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