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通过夹心酶联免疫吸附测定法中的一种灵敏的单克隆抗体对人γ干扰素进行定量。一种用于血清中测量的聚乙二醇修饰。

Human interferon-gamma quantified via a sensitive one-site monoclonal antibody in a sandwich ELISA. A PEG modification for measurement in serum.

作者信息

Berg K

机构信息

Interferon Laboratory, Panum Institute, Copenhagen, Denmark.

出版信息

APMIS. 1994 Jan;102(1):13-22. doi: 10.1111/j.1699-0463.1994.tb04840.x.

Abstract

A new, specific and sensitive one-site ELISA for precise quantification of human interferon-gamma (HuIFN-gamma) at low levels in 50% human serum samples has been developed. The assay is based on the assumption that biologically active HuIFN-gamma is present exclusively as a dimer. Thus, in contrast to previous reports, the ELISA is based on a single monoclonal antibody (MAb) which is used in two ways: as "catching" antibody and as HRPO-labelled conjugate. The sensitivity could be improved five-fold by addition of (NH4)2SO4 to the conjugate solution; the lowest detectable amount of HuIFN-gamma is < 0.5 mu/ml. Non-specific interactions were not seen in interferon samples taken from cultures, or samples diluted in ordinary media or 1% BSA. However, > 30% of the (serum) samples gave non-specific false-positive results when the method was applied to samples containing 50-100% human serum from different donors. The false signals were related to the donors but could-at the expense of the sensitivity which was reduced to 1 mu/ml-be abolished by PEG treatment of the (donor) serum samples.

摘要

已开发出一种新型、特异且灵敏的单位点酶联免疫吸附测定法(ELISA),用于精确量化50%人血清样本中低水平的人γ干扰素(HuIFN-γ)。该检测方法基于这样一种假设,即具有生物活性的HuIFN-γ仅以二聚体形式存在。因此,与先前的报道不同,该ELISA基于一种单克隆抗体(MAb),该抗体有两种使用方式:作为“捕获”抗体和作为辣根过氧化物酶(HRPO)标记的缀合物。通过向缀合溶液中添加硫酸铵((NH4)2SO4),灵敏度可提高五倍;HuIFN-γ的最低可检测量<0.5微克/毫升。在从培养物中获取的干扰素样本、在普通培养基或1%牛血清白蛋白(BSA)中稀释的样本中未观察到非特异性相互作用。然而,当该方法应用于含有来自不同供体的50%-100%人血清的样本时,超过30%的(血清)样本出现非特异性假阳性结果。这些假信号与供体有关,但通过对(供体)血清样本进行聚乙二醇(PEG)处理,可消除这些假信号,不过灵敏度会降至1微克/毫升。

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