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由EB病毒转化的B淋巴母细胞系产生的人IgG单克隆抗-D的半乳糖基化取决于培养方法,并影响Fc受体介导的功能活性。

Galactosylation of human IgG monoclonal anti-D produced by EBV-transformed B-lymphoblastoid cell lines is dependent on culture method and affects Fc receptor-mediated functional activity.

作者信息

Kumpel B M, Rademacher T W, Rook G A, Williams P J, Wilson I B

机构信息

International Blood Group Reference Laboratory, Bristol, UK.

出版信息

Hum Antibodies Hybridomas. 1994;5(3-4):143-51.

PMID:7756579
Abstract

Human monoclonal antibodies to the Rh D blood group antigen were produced by EBV-transformed B cell lines grown in serum-free medium in low density (LD) static cultures or high density (HD) hollow fiber bioreactors. Glycosylation analysis of the purified IgG was determined by the binding of anti-GlcNAc monoclonal antibody (GN7) and by analysis of oligosaccharides released by hydrazinolysis. The LD MAbs had only trace levels of agalactosyl oligosaccharides (G0), the major species (> 70%) being digalactosyl structures (G2). The HD MAbs, by contrast, contained about 10% G0 and relatively high levels (over 50%) of monogalactosyl (G1) oligosaccharides. beta 1-4 galactosyltransferase activity in the LD cell lines was similar to that found previously for other EBV-transformed B cell lines. The predominant oligosaccharides of an IgG3 anti-D, BRAD-3, contained bisecting N-acetylglucosamine. In functional assays with Fc receptor (Fc gamma R) positive effector cells, the highly galactosylated LD form of BRAD-3 was more active than the HD form in monocyte (Fc gamma RI) and K cell (Fc gamma RIII) mediated lysis of erythrocytes in ADCC assays, although these preparations showed no difference in Fc gamma RI-mediated rosette formation with U937 cells. One MAb, JAC10, was over 10-fold less active than two other IgG1 MAbs, 2B6 and BRAD-5, at mediating lysis of erythrocytes by Fc gamma RIII+ K cells; differences in sialylation may have contributed to this heterogeneity.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过在低密度(LD)静态培养的无血清培养基或高密度(HD)中空纤维生物反应器中培养的EBV转化B细胞系产生了针对Rh D血型抗原的人单克隆抗体。通过抗GlcNAc单克隆抗体(GN7)的结合以及对肼解释放的寡糖的分析来确定纯化IgG的糖基化分析。LD单克隆抗体仅含有痕量水平的无半乳糖寡糖(G0),主要种类(>70%)为二半乳糖结构(G2)。相比之下,HD单克隆抗体含有约10%的G0和相对较高水平(超过50%)的单半乳糖基(G1)寡糖。LD细胞系中的β1-4半乳糖基转移酶活性与先前在其他EBV转化B细胞系中发现的活性相似。一种IgG3抗-D抗体BRAD-3的主要寡糖含有平分型N-乙酰葡糖胺。在与Fc受体(FcγR)阳性效应细胞的功能测定中,在ADCC测定中,高度糖基化的LD形式的BRAD-3在单核细胞(FcγRI)和K细胞(FcγRIII)介导的红细胞裂解中比HD形式更具活性,尽管这些制剂在与U937细胞的FcγRI介导的玫瑰花结形成中没有差异。一种单克隆抗体JAC10在介导FcγRIII + K细胞对红细胞的裂解方面比另外两种IgG1单克隆抗体2B6和BRAD-5的活性低10倍以上;唾液酸化的差异可能导致了这种异质性。(摘要截断于250字)

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