首页> 美国卫生研究院文献>Clinical and Diagnostic Laboratory Immunology >Proteomic but Not Enzyme-Linked Immunosorbent Assay Technology Detects Amniotic Fluid Monomeric Calgranulins from Their Complexed Calprotectin Form
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Proteomic but Not Enzyme-Linked Immunosorbent Assay Technology Detects Amniotic Fluid Monomeric Calgranulins from Their Complexed Calprotectin Form

机译:蛋白质组学而非酶联免疫吸附测定技术可从其复杂的钙卫蛋白形式检测羊水单体钙粘蛋白

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摘要

Four proteomic biomarkers (human neutrophil peptide 1 [HNP1], HNP2 [defensins], calgranulin C [Cal-C], and Cal-A) characterize the fingerprint of intra-amniotic inflammation (IAI). We compared proteomic technology using surfaced-enhanced laser desorption-ionization-time of flight (SELDI-TOF) mass spectrometry to enzyme-linked immunosorbent assay (ELISA) for detection of these biomarkers. Amniocentesis was performed on 48 women enrolled in two groups: those with intact membranes (n = 27; gestational age [GA], 26.0 ± 0.8 weeks) and those with preterm premature rupture of the membranes (PPROM; n = 21; GA, 28.4 ± 0.9 weeks). Paired abdominal amniotic fluids (aAFs)-vaginal AFs (vAFs) were analyzed in PPROM women. Quantitative aspects of HNP1-3, Cal-C, Cal-A, and calprotectin (a complex of Cal-A with Cal-B) were assessed by ELISA. SELDI-TOF mass spectrometry tracings from 16/48 (33.3%) aAFs and 13/17 (88.2%) vAFs were consistent with IAI (three or four biomarkers present). IAI (by SELDI-TOF mass spectrometry) was associated with increased HNP1-3 and Cal-C measured by ELISA. However, immunoassays detected Cal-A in only 4 of the AFs even though its specific SELDI-TOF mass spectrometry peak was identified in 19/48 AFs. Calprotectin immunoreactivity was decreased in AFs retrieved from women with IAI (P = 0.01). In conclusion, IAI is associated with increased HNP1-3 levels. In the absence of isoform-specific ELISAs, mass spectrometry remains the only way to discriminate the HNP biomarker isoforms. Monomeric Cal-A is not reliably estimated by specific ELISA as it binds to Cal-B to form the calprotectin complex. Cal-C was reliably measured by SELDI-TOF mass spectrometry or specific ELISA.
机译:四种蛋白质组生物标志物(人中性粒细胞肽1 [HNP1],HNP2 [defensins],钙粒蛋白C [Cal-C]和Cal-A)表征羊膜内炎症(IAI)的指纹。我们比较了使用表面增强激光解吸-电离飞行时间(SELDI-TOF)质谱与酶联免疫吸附测定(ELISA)的蛋白质组学技术来检测这些生物标记物。分为两组的48名妇女进行了羊膜穿刺术:胎膜完整的妇女(n = 27;胎龄[GA],26.0±0.8周)和胎膜早破的妇女(PPROM; n = 21; GA,28.4) ±0.9周)。在PPROM妇女中分析了成对的腹部羊水(aAFs)-阴道AFs(vAFs)。通过ELISA评估了HNP1-3,Cal-C,Cal-A和钙卫蛋白(Cal-A与Cal-B的复合物)的定量方面。来自16/48(33.3%)aAF和13/17(88.2%)vAF的SELDI-TOF质谱示踪与IAI一致(存在三个或四个生物标记)。 IAI(通过SELDI-TOF质谱分析)与HNP1-3和ELISA检测的Cal-C升高有关。但是,即使在19/48个AF中发现了其特定的SELDI-TOF质谱峰,免疫分析也仅在4个AF中检测到了Cal-A。从患有IAI的女性中获取的AF中钙卫蛋白的免疫反应性降低(P = 0.01)。总之,IAI与HNP1-3水平升高有关。在没有同工型特异性ELISA的情况下,质谱分析仍然是区分HNP生物标志物同工型的唯一方法。单体Cal-A无法通过特异性ELISA可靠地评估,因为它与Cal-B结合形成钙卫蛋白复合物。通过SELDI-TOF质谱或特异性ELISA可靠地测量了Cal-C。

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