Features of N-Glycosylation of Immunoglobulins from Knockout Pig Models

Marjorie Buist, Emy Komatsu, Paul G. Lopez, L. Girard, Edward D Bodnar, A. Salama, D. Sachs, C. Galli, A. Perota, S. Conchon, Jean-Paul Judor, J. Concordet, G. Lazzari, J. Soulillou, H. Perreault
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引用次数: 3

Abstract

For the first time, the N-glycosylation patterns of immunoglobulin G (IgGs) isolated from the serum of two varieties of knockout pigs (lacking N-glycolylneuraminic acid (Neu5Gc) and/or α 1,3 galactose) were examined for the presence of potential glycan xenoantigens and compared to N-glycosylation patterns obtained for wild-type (WT) pig IgGs. Glycopeptide analysis was chosen over glycan release, as protein-A eluates from pig serum may contain IgA and IgM as shown previously. The experiments focused on the analysis of tryptic glycopeptides EEQFNSTYR and AEQFNSTYR from IgGs, and excluded IgA and IgM, in which N-glycosylated peptides have different sequences and masses. WT pig IgG glycopeptides showed the presence of N-glycolylneuraminic acid (Neu5Gc) and absence of N-acetylneuraminic acid (Neu5Ac). Released glycans from the protein-A eluate, however, showed the presence of both types of sialic acids, allowing Neu5Ac to be attributed to IgA and/or IgM. The WT IgG samples also showed the presence of glycans that could by composition have been α-galactosylated, but treatments with α- and β-galactosidases produced inconclusive results as to the linkage nature of the terminal Gal residues. Single knockout (α-Gal transferase) pig IgG was shown to contain Neu5Gc residues, and there was a definite absence of α-Gal. Double knockout pigs (DKO for α-Gal transferase and cytidine monophosphate-A-acetylneuraminic acid hydroxylase (CMAH)) showed the definite absence of α-Gal and Neu5Gc. Instead of the latter, Neu5Ac residues were observed. Further investigation into the sialylation patterns of WT and DKO pig IgGs consisted of esterifying the glycopeptides to allow the detection and differentiation of α-2,3 and α-2,6 sialic acid-galactose linkages. Fucosylation levels were also compared between IgG species.
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敲除猪免疫球蛋白n -糖基化特征
本文首次检测了两种基因敲除猪(缺乏n -糖基神经氨酸(Neu5Gc)和/或α 1,3半乳糖)血清中分离的免疫球蛋白G (IgGs)的n -糖基化模式是否存在潜在的聚糖异种抗原,并与野生型(WT)猪igg的n -糖基化模式进行了比较。我们选择糖肽分析而不是多糖释放,因为猪血清中的蛋白a洗脱物可能含有IgA和IgM,如前所述。实验重点分析IgGs中的色氨酸肽EEQFNSTYR和AEQFNSTYR,排除了其中n -糖基化肽序列和质量不同的IgA和IgM。WT猪IgG糖肽中存在n -糖基神经氨酸(Neu5Gc),不存在n -乙酰基神经氨酸(Neu5Ac)。然而,从蛋白a洗脱液中释放的聚糖显示了两种类型唾液酸的存在,允许Neu5Ac归因于IgA和/或IgM。WT IgG样品也显示存在可以通过组成被α-半乳糖化的聚糖,但α-和β-半乳糖苷酶处理对末端Gal残基的连锁性质产生不确定的结果。单敲除(α-Gal转移酶)猪IgG含有Neu5Gc残基,α-Gal明显缺失。双敲除猪(α-Gal转移酶和胞苷单磷酸-a -乙酰神经氨酸羟化酶(CMAH)的DKO)显示α-Gal和Neu5Gc的明确缺失。而不是后者,观察到Neu5Ac残基。对WT和DKO猪igg唾液化模式的进一步研究包括糖肽的酯化,以检测和区分α-2,3和α-2,6唾液酸-半乳糖键。还比较了不同IgG种间的聚焦化水平。
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