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通过EBV转化和B淋巴细胞的抗原特异性选择获得的人单克隆抗体。

Human monoclonals from antigen-specific selection of B lymphocytes and transformation by EBV.

作者信息

Casali P, Inghirami G, Nakamura M, Davies T F, Notkins A L

出版信息

Science. 1986 Oct 24;234(4775):476-9. doi: 10.1126/science.3020687.

Abstract

Hybridoma technology has made it possible to prepare monoclonal antibodies with the use of murine lymphocytes. Attempts to extend this technology to the human level, however, have met with difficulties. A method has been developed for making human monoclonal antibodies of predetermined specificity. Biotinylated antigens (human thyroglobulin or tetanus toxoid) were incubated with human B lymphocytes from peripheral blood. The lymphocytes to which the antigens bound were selected by fluorescence-activated cell sorting. Positively selected (high fluorescence) and negatively selected (low fluorescence) cells were then transformed with Epstein-Barr virus (EBV) and grown in microculture wells. All wells from the positively selected fraction produced antigen-specific antibody (95 to 1800 nanogram-equivalents per milliliter), whereas fewer than 6% of the wells from negatively selected fraction made any detectable antibody (less than 10 nanogram-equivalents per milliliter). When the positively selected EBV-transformed cells were cultured in limiting dilution, clones were obtained that made antigen-specific monoclonal antibodies. By this method, monoclonal antibodies to both foreign antigens and autoantigens can be prepared from the normal human B-cell repertoire.

摘要

杂交瘤技术使得利用鼠淋巴细胞制备单克隆抗体成为可能。然而,将该技术扩展至人类水平的尝试却遇到了困难。现已开发出一种制备具有预定特异性的人单克隆抗体的方法。将生物素化抗原(人甲状腺球蛋白或破伤风类毒素)与外周血中的人B淋巴细胞一起孵育。通过荧光激活细胞分选来选择结合了抗原的淋巴细胞。然后,用爱泼斯坦 - 巴尔病毒(EBV)转化阳性选择(高荧光)和阴性选择(低荧光)的细胞,并在微量培养孔中培养。阳性选择部分的所有孔均产生了抗原特异性抗体(每毫升95至1800纳克当量),而阴性选择部分的孔中只有不到6%产生了任何可检测到的抗体(每毫升少于10纳克当量)。当对阳性选择的EBV转化细胞进行有限稀释培养时,获得了产生抗原特异性单克隆抗体的克隆。通过这种方法,可以从正常人B细胞库中制备针对外来抗原和自身抗原的单克隆抗体。

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