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首页> 外文期刊>The Journal of biological chemistry >Fc γ receptor IIIa/CD16a processing correlates with the expression of glycan-related genes in human natural killer cells
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Fc γ receptor IIIa/CD16a processing correlates with the expression of glycan-related genes in human natural killer cells

机译:Fcγ受体IIIA / CD16A处理与人类天然杀伤细胞中甘草相关基因的表达相关

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Many therapeutic monoclonal antibodies require binding to Fc γ receptors (FcγRs) for full effect and increasing the binding affinity increases efficacy. Preeminent among the five activating human FcγRs is FcγRIIIa/CD16a expressed by natural killer (NK) cells. CD16a is heavily processed, and recent reports indicate that the composition of the five CD16a asparagine(N)-linked carbohydrates (glycans) impacts affinity. These observations indicate that specific manipulation of CD16a N-glycan composition in CD16a-expressing effector cells including NK cells may improve treatment efficacy. However, it is unclear if modifying the expression of select genes that encode processing enzymes in CD16a-expressing effector cells is sufficient to affect N-glycan composition. We identified substantial processing differences using a glycoproteomics approach by comparing CD16a isolated from two NK cell lines, NK92 and YTS, with CD16a expressed by HEK293F?cells and previous reports of CD16a from primary NK cells. Gene expression profiling by RNA-Seq and qRT-PCR revealed expression levels for glycan-modifying genes that correlated with CD16a glycan composition. These results identified a high degree of variability between the processing of the same human protein by different human cell types. N-glycan processing correlated with the expression of glycan-modifying genes and thus explained the substantial differences in CD16a processing by NK cells of different origins.
机译:许多治疗性单克隆抗体需要与Fcγ受体(FcγRS)结合以进行全效果,并增加结合亲和力增加功效。五种激活人FCγRS的卓越是由天然杀伤剂(NK)细胞表达的FCγRIIIA/ CD16a。 CD16a受到严重处理,最近的报告表明,五个CD16A天冬酰胺(N) - 链接碳水化合物(聚糖)的组成影响了亲和力。这些观察结果表明,在包括NK细胞的CD16A表达效应细胞中的CD16A N-聚糖组合物的具体操纵可以改善治疗效果。然而,目前尚不清楚修饰编码CD16A表达的效应细胞中的加工酶的选择基因的表达是否足以影响N-聚糖组合物。我们通过将CD16A与来自HEK293F的CD16A与HEK293Fα细胞表达的CD16a与来自主NK细胞的CD16a表达的CD16a进行比较,使用糖蛋白质方法进行了大量的处理差异。通过RNA-SEQ和QRT-PCR的基因表达分析揭示了与CD16a聚糖组合物相关的甘油改性基因的表达水平。这些结果通过不同的人体细胞类型鉴定了相同人类蛋白质的加工之间的高度可变性。 N-聚糖处理与聚糖改性基因的表达相关,从而解释了不同起源的NK细胞CD16a处理的显着差异。

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