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对转基因兔乳汁中产生的人活化凝血因子VII进行N-糖基化和O-糖基化分析。

N-/O-glycosylation analysis of human FVIIa produced in the milk of transgenic rabbits.

作者信息

Chevreux Guillaume, Faid Valegh, Scohyers Jean-Marc, Bihoreau Nicolas

机构信息

Analytical Department, LFB Biotechnologies, 3 Avenue des Tropiques, Les Ulis, 91942 Courtaboeuf, France.

出版信息

Glycobiology. 2013 Dec;23(12):1531-46. doi: 10.1093/glycob/cwt085. Epub 2013 Oct 2.

Abstract

Human coagulation factor VIIa is a glycoprotein that promotes haemostasis through activation of the coagulation cascade extrinsic pathway. Most haemophilia A/B patients with inhibitors are treated by injection of plasma-derived or recombinant FVIIa. The use of recombinant products raises questions about the ability of the host cell to produce efficiently post-translationally modified proteins. Glycosylation is especially critical considering that it can modulate protein safety and efficacy. The present paper reports the N-/O-glycosylation pattern of a new recombinant human factor VIIa expressed in the mammary glands of transgenic rabbits. Glycosylation was investigated by chromatography and advanced mass spectrometry techniques for glycan identification and quantitation. Mass spectrometry (MS)/MS analyses were performed to confirm the glycan structures as well as the position and branching of specific monosaccharides or substituents. The two N-glycosylation sites were found to be fully occupied mostly by mono- and bi-sialylated biantennary complex-type structures, the major form being A(2)G(2)S(1). Some oligomannose/hybrid structures were retrieved in lower abundance, the major ones being GlcNAcα1,O-phosphorylated at the C6-position of a Man residue (Man-6-(GlcNAcα1,O-)phosphate motif) as commonly observed on lysosomal proteins. No immunogenic glycotopes such as Galili (Galα1,3Gal) and HD antigens (N-glycolylneuraminic acid (NeuGc)) were detected. Concerning O-glycosylation, the product exhibited O-fucose and O-glucose-(xylose)(0, 1, 2) motifs as expected. The N-glycosylation consistency was also investigated by varying production parameters such as the period of lactation, the number of consecutive lactations and rabbit generations. Results show that the transgenesis technology is suitable for the long-term production of rhFVIIa with a reproducible glycosylation pattern.

摘要

人凝血因子VIIa是一种糖蛋白,通过激活凝血级联外源性途径促进止血。大多数患有抑制剂的甲型/乙型血友病患者通过注射血浆源性或重组FVIIa进行治疗。重组产品的使用引发了关于宿主细胞有效生产翻译后修饰蛋白能力的问题。考虑到糖基化可以调节蛋白质的安全性和有效性,其尤为关键。本文报道了在转基因兔乳腺中表达的一种新型重组人因子VIIa的N-/O-糖基化模式。通过色谱法和先进的质谱技术对糖基化进行研究,以鉴定和定量聚糖。进行质谱(MS)/MS分析以确认聚糖结构以及特定单糖或取代基的位置和分支。发现两个N-糖基化位点大多被单唾液酸化和双唾液酸化的双天线复合型结构完全占据,主要形式为A(2)G(2)S(1)。一些低聚甘露糖/杂合结构以较低丰度被检测到,主要的是在溶酶体蛋白上常见的在Man残基的C6位被GlcNAcα1,O-磷酸化(Man-6-(GlcNAcα1,O-)磷酸基序)。未检测到免疫原性糖基表位,如Galili(Galα1,3Gal)和HD抗原(N-羟乙酰神经氨酸(NeuGc))。关于O-糖基化,该产品表现出预期的O-岩藻糖和O-葡萄糖-(木糖)(0, 1, 2)基序。还通过改变生产参数,如哺乳期、连续泌乳次数和兔代次,研究了N-糖基化的一致性。结果表明,转基因技术适用于长期生产具有可重复糖基化模式的重组人FVIIa。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8a6f/3816631/62b09551cb9d/cwt08501.jpg

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