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可与细胞抗原发生反应的人单克隆抗体的产生。

Generation of human monoclonal antibodies reactive with cellular antigens.

作者信息

Cote R J, Morrissey D M, Houghton A N, Beattie E J, Oettgen H F, Old L J

出版信息

Proc Natl Acad Sci U S A. 1983 Apr;80(7):2026-30. doi: 10.1073/pnas.80.7.2026.

Abstract

Human lymphocytes from lymph node, peripheral blood, spleen, and tumor specimens have been fused with the LICR-LON-HMy2 (LICR-2) or SKO-007 human cell lines or the NS-1 mouse myeloma line. Over 75 fusions with the three myeloma-lymphoblastoid lines have been performed. Several factors appeared to improve the fusion outcome, including maintenance of the myeloma-lymphoblastoid lines in logarithmic phase growth at greater than or equal to 95% viability, a delay of 24 hr in the introduction of aminopterin to the fused cells, and preselection of the fetal calf serum used in the medium. For a given number of lymphocytes, fusions with NS-1 produced 5-20 times more clones than fusions with LICR-2 or SKO-007, and LICR-2 produced 4 times as many clones as SKO-007. The percentage of clones secreting human immunoglobulin, the range of immunoglobulin production, and the proportion of IgM, IgA, and IgG secretors were comparable for clones derived from the three myeloma-lymphoblastoid lines. Stable Ig-secreting clones were isolated with approximately equal frequency from LICR-2 and NS-1 fusions. A number of stable clones producing human monoclonal antibodies reacting with cell-surface, cytoplasmic, or nuclear antigens have been isolated from tumor-bearing patients and normal individuals. A surface antigenic system present on normal and malignant cells has been defined with a human monoclonal antibody derived from a patient with breast cancer. Techniques for producing human monoclonal antibody now appear to be sufficiently advanced to initiate a serological dissection of the humoral immune response to cancer.

摘要

来自淋巴结、外周血、脾脏和肿瘤标本的人淋巴细胞已与LICR-LON-HMy2(LICR-2)或SKO-007人细胞系或NS-1小鼠骨髓瘤细胞系融合。已进行了超过75次与这三种骨髓瘤-淋巴母细胞系的融合。有几个因素似乎能改善融合结果,包括将骨髓瘤-淋巴母细胞系维持在对数生长期且活力大于或等于95%,在融合细胞中延迟24小时引入氨基蝶呤,以及对培养基中使用的胎牛血清进行预选。对于给定数量的淋巴细胞,与NS-1融合产生的克隆数比与LICR-2或SKO-007融合产生的克隆数多5至20倍,且LICR-2产生的克隆数是SKO-007的4倍。对于源自这三种骨髓瘤-淋巴母细胞系的克隆,分泌人免疫球蛋白的克隆百分比、免疫球蛋白产生范围以及IgM、IgA和IgG分泌者的比例相当。从LICR-2和NS-1融合物中以大致相同的频率分离出稳定的Ig分泌克隆。已从荷瘤患者和正常个体中分离出许多产生与人细胞表面、细胞质或核抗原反应的人单克隆抗体的稳定克隆。用一名乳腺癌患者来源的人单克隆抗体定义了正常细胞和恶性细胞上存在的一种表面抗原系统。现在,生产人单克隆抗体的技术似乎已足够先进,能够启动对癌症体液免疫反应的血清学剖析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2c11/393745/b059b34127cf/pnas00633-0250-a.jpg

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