首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Radioimmunochemical measurement of the transferrin receptor in human trophoblast and reticulocyte membranes with a specific anti-receptor antibody.
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Radioimmunochemical measurement of the transferrin receptor in human trophoblast and reticulocyte membranes with a specific anti-receptor antibody.

机译:用特定的抗受体抗体对人体滋养细胞和网织红细胞膜中转铁蛋白受体进行放射免疫化学测定。

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摘要

A radioimmunoassay was developed to directly assay the presence of transferrin receptors in human tissues. Antisera developed in a goat against purified human placental transferrin binding protein was purified by fractional sodium sulfate precipitation and adsorption against Sepharose-bound transferrin to remove trace anti-transferrin activity. The antisera immunoprecipitates a Mr 94,000 peptide on 125I-iodinated syncytial trophoblast membranes from placentae. This polypeptide has been identified previously as the transferrin binding protein of the placenta [Wada, H. G., Hass, P. E. & Sussman, H. H. (1979) J. Biol. Chem. 254, 12629-12635]. A standard curve using purified 125I-iodinated placental transferrin receptor and various amounts of the purified noniodinated receptor is sensitive from 5 to 900 ng. A reticulocyte-enriched membrane ghost preparation (5% reticulocyte) gives a value of 9.5 micrograms of receptor per mg of protein. Normal erythrocyte membrane ghosts show binding (0.57 micrograms of receptor per mg of protein) proportional to the amount of reticulocytes normally present in blood (0.5-1.0%). In other tissues in which the transferrin receptor binding has been reported, purified syncytial trophoblastic membranes are found to have 34.5 micrograms of receptor per mg of protein, and BeWo cells, a choriocarcinoma cell line, are found to have 15.7 micrograms of receptor per mg of protein. In contrast, normal breast tissue, which has no demonstrated transferrin binding, contains only 0.18 micrograms of receptor per mg of protein by this method.
机译:开发了一种放射免疫测定法以直接测定人体组织中转铁蛋白受体的存在。通过部分硫酸钠沉淀并吸附针对琼脂糖结合的转铁蛋白的吸附来纯化山羊中针对纯化的人胎盘转铁蛋白结合蛋白的抗血清,以去除痕量的抗转铁蛋白活性。该抗血清使来自胎盘的125I碘化合胞体滋养细胞膜上的94,000 Mr肽免疫沉淀。该多肽先前已被鉴定为胎盘的运铁蛋白结合蛋白[Wada,H.G.,Hass,P.E。&Sussman,H.H。(1979)J.Biol.Chem.Soc。,1992,5,1897]。化学254,12629-12635]。使用纯化的125 I-碘化的胎盘运铁蛋白受体和各种量的纯化的非碘化受体的标准曲线在5到900 ng范围内敏感。富含网状细胞的膜重影制剂(5%网状细胞)的值为每毫克蛋白质9.5微克受体。正常的红细胞膜重影显示出与血液中正常存在的网织红细胞数量成比例(0.5-1.0%)的结合(每毫克蛋白质0.57微克受体)。在其他已经报道了转铁蛋白受体结合的组织中,发现纯化的合胞体滋养层膜每毫克蛋白具有34.5微克受体,绒毛膜癌细胞系BeWo细胞每毫克蛋白具有15.7微克受体。蛋白。相反,通过这种方法,未​​证明转铁蛋白结合的正常乳腺组织每毫克蛋白质仅含有0.18微克受体。

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