Houghton A N, Brooks H, Cote R J, Taormina M C, Oettgen H F, Old L J
J Exp Med. 1983 Jul 1;158(1):53-65. doi: 10.1084/jem.158.1.53.
This study represents an initial attempt to analyze the humoral immune reactions of patients with malignant melanoma by hybridoma methodology. Using lymphocytes from regional lymph nodes, peripheral blood and tumor infiltrates, 158 fusions were performed with SKO-007 (human myeloma line), LICR-LON-HMy2 (LICR-2), GM 4672 (human lymphoblastoid lines), or NS-1 (mouse myeloma line). Fusion of lymph node lymphocytes with NS-1 resulted in a 3-4 times higher frequency of clones than fusion with LICR-2, and a 10 times higher frequency than fusion with SKO-007 or GM 4672. In the case of peripheral blood lymphocytes, fusion with NS-1 gave greater than 25 times higher frequency of clones than fusion with LICR-2 or SKO-007. Production of human mu, gamma, or alpha heavy chains was detected in 50-80% of wells containing growing clones, and the levels of immunoglobulin ranged from 0.3 micrograms to 40 micrograms/ml. NS-1-derived clones could be easily subcultured, while LICR-2 and SKO-007 clones grew more slowly on subculturing. In this study, Ig secretion appeared to be a more stable property of LICR-2-derived clones than NS-1-derived clones. A panel of 20 human cancer cell lines was used to screen 771 Ig-secreting cultures for antibody to cell surface or intracellular antigens. Reactivity with cell surface antigens was found infrequently (6 cultures), whereas reactivity with intracellular antigens was more common (27 cultures). A new cell surface antigen with properties of a glycolipid was defined with an IgM monoclonal antibody secreted by a tetraploid cell derived from a fusion of LICR-2 with lymphocytes from the axillary lymph node of a patient with melanoma. The hybrid cell line has been subcloned four times and secretes 5 micrograms IgM/ml. The antigen detected by this IgM antibody was found on 5 of 23 melanoma cell lines and 12 of 30 epithelial cancer cell lines. No reactions were found with 11 cultures derived from normal cells. Stable cell lines secreting human antibody that detected nuclei, nucleoli, cytoskeletal elements, Golgi complex, or other cytoplasmic components were also isolated in this study. One of these antibodies detected an intracellular antigen that is restricted to cells of neuroectodermal derivation, and a second antibody reacted primarily with cells of epithelial origin. Using these methods to isolate and analyze human monoclonal antibody, it should now be possible to define the repertoire of the humoral immune response to melanoma.
本研究是通过杂交瘤技术分析恶性黑色素瘤患者体液免疫反应的初步尝试。利用来自区域淋巴结、外周血和肿瘤浸润组织的淋巴细胞,分别与SKO-007(人骨髓瘤细胞系)、LICR-LON-HMy2(LICR-2)、GM 4672(人淋巴母细胞系)或NS-1(小鼠骨髓瘤细胞系)进行了158次融合。淋巴结淋巴细胞与NS-1融合产生的克隆频率比与LICR-2融合高3 - 4倍,比与SKO-007或GM 4672融合高10倍。对于外周血淋巴细胞,与NS-1融合产生的克隆频率比与LICR-2或SKO-007融合高25倍以上。在含有生长克隆的50 - 80%的孔中检测到了人μ、γ或α重链的产生,免疫球蛋白水平在0.3微克/毫升至40微克/毫升之间。源自NS-1的克隆易于传代培养,而LICR-2和SKO-007克隆传代培养时生长较慢。在本研究中,LICR-2衍生的克隆的Ig分泌似乎比NS-1衍生的克隆更稳定。使用一组20种人类癌细胞系对771种分泌Ig的培养物进行筛选,以检测其针对细胞表面或细胞内抗原的抗体。很少发现与细胞表面抗原的反应(6种培养物),而与细胞内抗原的反应更为常见(27种培养物)。用LICR-2与一名黑色素瘤患者腋窝淋巴结淋巴细胞融合产生的四倍体细胞分泌的IgM单克隆抗体定义了一种具有糖脂特性的新细胞表面抗原。该杂交细胞系已进行了四次亚克隆,分泌5微克/毫升的IgM。这种IgM抗体检测到的抗原在23种黑色素瘤细胞系中的5种以及30种上皮癌细胞系中的12种上被发现。在11种源自正常细胞的培养物中未发现反应。在本研究中还分离出了分泌能检测细胞核、核仁、细胞骨架成分、高尔基体或其他细胞质成分的人抗体的稳定细胞系。其中一种抗体检测到一种仅限于神经外胚层来源细胞的细胞内抗原,另一种抗体主要与上皮来源的细胞反应。利用这些方法分离和分析人单克隆抗体,现在应该能够确定针对黑色素瘤的体液免疫反应谱。
