猪 B4GALNT2 和 B4GALNT2 样蛋白的酶学比较和表达模式

Anjing Zhang, Z. Zhong, Dengke Pan, Peidong Yang, Shuqi Yang, Jideng Ma, Tingting Luo, Li Chen, Jinwei Zhang, Jing Sun, Jiaxiang Du, K. Long, Mingzhou Li, Lu Lu
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引用次数: 0

摘要

目的制备人Sd(a)抗原的最后一步是由β -1,4- n -乙酰半乳糖胺转移酶2 (B4GALNT2)催化。这是通过-1,4链将n -乙酰半乳糖胺残基添加到亚末端半乳糖残基上,该半乳糖残基已被-2,3链唾液酸取代。Cad抗原产生的最后阶段也由B4GALNT2催化。敲除猪B4GALNT2基因可降低人血清抗体与猪细胞的结合,从而大大降低临床异种移植试验中的免疫排斥反应。有趣的是,LOC110255214基因区域(以下简称B4GALNT2-like)在我们之前的工作中显示出与猪基因组中的B4GALNT2基因高度相似,但B4GALNT2-like是否与B4GALNT2具有相似的生物学特性仍有待阐明,B4GALNT2-like是否在异种移植中具有潜在的免疫基因仍有待确定。方法比较B4GALNT2样蛋白和B4GALNT2在巴马猪组织中的表达模式。结果B4GALNT2-like在十二指肠的表达明显高于B4GALNT2,而在心脏、脾脏、肺、肾脏的表达明显低于B4GALNT2。应用大肠杆菌重组表达,从1个 L培养中分别获得B4GALNT2和B4GALNT2样蛋白768和1,300 μg。利用表达的重组蛋白对两种蛋白的酶活性进行测定和比较。结论酶促实验显示B4GALNT2-like与B4GALNT2具有相当的催化活性(58.7 % B4GALNT2),解决了B4GALNT2-like是否为一种新的免疫排斥基因的重要问题。
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Enzymatic comparison and expression pattern of pig B4GALNT2 and B4GALNT2-like proteins
Abstract Objectives The final step in the production of the human Sd(a) antigen is catalyzed by beta-1,4-N-acetyl-galactosamine transferase 2 (B4GALNT2). This is done by adding a N-acetylgalactosamine residue via a beta-1,4 linkage to a subterminal galactose residue that has been substituted with an alpha-2,3-linked sialic acid. The final stage of the production of the Cad antigen is also catalyzed by B4GALNT2. Knocking out pig B4GALNT2 gene decreased human serum antibodies binding to pig cells, which greatly reduces the immunological rejection in clinical xenotransplantation trials. Interestingly, gene region LOC110255214 (hereafter named B4GALNT2-like) showed high similarity with the B4GALNT2 gene in the pig genome in our previous work, but whether B4GALNT2-like shares similar biological properties like B4GALNT2 remains to be elucidated, whether B4GALNT2-like is a potential immune gene in xenotransplantation remains to be determined. Methods In this study, we compared the tissue expression pattern of B4GALNT2-like and B4GALNT2 in Bama pigs. Results We found the expression of B4GALNT2-like was significantly higher in the duodenum, but lower in the heart, spleen, lung, kidney, comparing to B4GALNT2. Applied the Escherichia coli recombinant expression, we obtained 768 and 1,300 μg protein for B4GALNT2 and B4GALNT2-like from 1 L culture, respectively. Using the expressed recombinant proteins, the enzymatic activity of the two proteins was determined and compared. Conclusions The enzymatic assay showed that B4GALNT2-like has comparable catalytic activity with B4GALNT2 (58.7 % of B4GALNT2), addressing an important question whether B4GALNT2-like is a new immunological rejection gene.
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