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Development of an assay for a biomarker of pregnancy and early fetal loss.

机译:妊娠和早期胎儿丢失的生物标志物检测方法的开发。

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摘要

Human chorionic gonadotropin (hCG) is a glycoprotein hormone, secreted by the syncytiotrophoblast cells of the fertilized ovum, that enters the maternal circulation at the time of endometrial implantation. It is composed of two nonidentical subunits; alpha and beta, with molecular weights of 14 kD and 23 kD, respectively. Its alpha subunit is identical in primary structure to its glycoprotein homologs, luteinizing hormone (LH), follicle-stimulating hormone (FSH), and thyroid-stimulating hormone (TSH). Human chorionic gonadotropin binds to the same receptor as hLH and displays the same biological response, namely, to stimulate the declining function of the corpus luteum to produce progestins and estrogen late in the menstrual cycle. The differences in the structures of hCG and hLH have been exploited to develop antibodies that can measure hCG specifically in the presence of hLH. Two-site antibody binding assays have been developed, based on a surface immunological concept of hCG epitopes, that involve four distinct regions to which antibodies against hCG can bind simultaneously. Antibody cooperative effects, in conjunction with kinetic advantages derived from the concentration factors by use of the sandwich assay technique (immunoradiometric assay, IRMA), have enabled development of extremely sensitive and specific measurement protocols for urinary hCG. The assay described herein permits the detection of pregnancy on an average 25.4 days after the first day of the preceding menses, as opposed to 29.5 days for conventional radioimmunoassay techniques. In addition, the greater sensitivity and specificity of this assay method has permitted the detection of episodes of fetal loss not detected by radioimmunoassay of urine specimens. A large scale epidemiological study is in progress using this assay technique as a way to identify pregnancies that are lost before becoming clinically apparent. This methodology provides a valuable tool for the determination of the rate of early fetal loss.
机译:人绒毛膜促性腺激素(hCG)是一种糖蛋白激素,由受精卵的合体滋养层细胞分泌,在子宫内膜植入时进入母体循环。它由两个不同的亚单元组成; α和β,分子量分别为14 kD和23 kD。它的α亚基的一级结构与其糖蛋白同源物,促黄体激素(LH),促卵泡激素(FSH)和促甲状腺激素(TSH)相同。人绒毛膜促性腺激素与hLH结合到同一受体上,并显示出相同的生物学反应,即在月经周期后期刺激黄体的功能下降以产生孕激素和雌激素。已利用hCG和hLH结构上的差异来开发可在hLH存在下特异性测量hCG的抗体。基于hCG表位的表面免疫学概念,已经开发了两点抗体结合测定法,其涉及针对hCG的抗体可以同时结合的四个不同区域。抗体的协同作用,以及通过使用夹心测定技术(免疫放射测定,IRMA)从浓度因子中获得的动力学优势,已为尿hCG的开发提供了极为灵敏和特异的测量方案。与常规放射免疫分析技术的29.5天相比,本文所述的分析方法可在前一次月经的第一天后平均25.4天检测到妊娠。另外,这种测定方法的更高的灵敏度和特异性使得能够检测出通过尿液标本的放射免疫测定未检测到的胎儿丢失发作。使用该测定技术的大规模流行病学研究正在进行中,以作为在临床上变得明显之前鉴定丢失的妊娠的一种方法。这种方法为确定早期胎儿流失率提供了宝贵的工具。

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