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爱泼斯坦-巴尔病毒诱导产生抗体的细胞系

Induction of antibody-producing cell lines by Epstein-Barr virus.

作者信息

Viallat J R, Kourilsky F M

出版信息

Pathol Biol (Paris). 1982 Apr;30(4):232-42.

PMID:6283460
Abstract

This work makes a critical evaluation of EBV transformation as a tool for establishing human antibody producing lines. Since Steinitz et al. described the technique in 1977, at least 9 lymphoid cell lines with predetermined specificities have been reported with activity against NNP, TNP, A-CHO, phosphorylcholine, human Ig, Rh-D antigen and tetanus toxoid. Most successful attempts were based on the choice of immune donors and on the adequate selection of peripheral antigen-specific B cells with antigen-coated erythrocytes. When lines were established, a further selection of antigen-specific lymphoblastoid cells using several steps of rosetting or cloning proved to be necessary, in order to get mono- or oligoclonal lines, and thus to maintain an antibody production for a prolonged period (up to 18 months). Secretion ranged from 0.1 to 16 micrograms antibody per ml, depending on the lines. Two of the antibodies produced are used as biological reagents. When compared to hybridomas, EBV transformed lines have the disadvantage of a lower colony forming efficiency, and usually a lower level of antibody secretion. On the other hand, if fusion of EBV induced lymphoblastoid cell lines proves to be possible with human myeloma lines and results in the creation of hybridomas, EBV transformation might reveal a useful technique to raise minute amounts of antigen specific cells to the amount of cells required for the fusion techniques.

摘要

这项工作对EBV转化作为建立人抗体产生细胞系的一种工具进行了批判性评估。自1977年Steinitz等人描述该技术以来,至少已有9种具有预定特异性的淋巴样细胞系被报道,它们对NNP、TNP、A-CHO、磷酸胆碱、人Ig、Rh-D抗原和破伤风类毒素具有活性。大多数成功的尝试基于免疫供体的选择以及用抗原包被的红细胞对外周抗原特异性B细胞进行适当选择。当建立细胞系时,为了获得单克隆或寡克隆细胞系,并因此长时间维持抗体产生(长达18个月),证明有必要使用几步玫瑰花结形成或克隆对抗原特异性淋巴母细胞样细胞进行进一步选择。抗体分泌量为每毫升0.1至16微克,具体取决于细胞系。所产生的两种抗体用作生物试剂。与杂交瘤相比,EBV转化细胞系的缺点是集落形成效率较低,且通常抗体分泌水平较低。另一方面,如果EBV诱导的淋巴母细胞样细胞系与人类骨髓瘤细胞系的融合被证明是可行的,并导致杂交瘤的产生,那么EBV转化可能会成为一种有用的技术,将微量的抗原特异性细胞增加到融合技术所需的细胞数量。

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