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Sequence properties of GPI-anchored proteins near the omega-site: constraints for the polypeptide binding site of the putative transamidase

机译:GPI锚定蛋白质在欧米茄位点附近的序列特性:假定的转酰胺酶的多肽结合位点的限制

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摘要

Glycosylphosphatidylinositol (GPI) anchoring is a common post-translational modification of extracellular eukaryotic proteins, Attachment of the GPI moiety to the carboxyl terminus (omega-site) of the polypeptide occurs after proteolytic cleavage of a C-terminal propeptide. In this work, the sequence pattern for GPI-modification was analyzed in terms of physical amino acid properties based on a database analysis of annotated proprotein sequences. In addition to a refinement of previously described sequence signals, we report conserved sequence properties in the regions omega - 11...omega - 1 and omega + 4...omega + 5. We present statistical evidence for volume-compensating residue exchanges with respect to the positions omega - 1...omega + 2. Differences between protozoan and metazoan GPI-modification motifs consist mainly in variations of preferences to amino acid types at the positions near the omega-site and in the overall motif length. The variations of polypeptide substrates are exploited to suggest a model of the polypeptide binding site of the putative transamidase, the enzyme catalyzing the GPI-modification. The volume of the active site cleft accommodating the four residues omega - 1...omega + 2 appears to be similar to 540 Angstrom(3). [References: 31]
机译:糖基磷脂酰肌醇(GPI)锚定是细胞外真核蛋白质的常见翻译后修饰,GPI部分与多肽的羧基末端(ω位)的连接发生在C端前肽的蛋白水解后。在这项工作中,基于注释的前蛋白序列的数据库分析,根据物理氨基酸特性分析了GPI修饰的序列模式。除了改进先前描述的序列信号外,我们还报告了omega-11 ... omega-1和omega + 4 ... omega + 5区域中的保守序列特性。关于ω-1 ... omega + 2的位置。原生动物和后生动物的GPI修饰基序之间的差异主要在于在ω位附近的位置和整个基序长度上对氨基酸类型的偏好变化。利用多肽底物的变化来暗示推定的酰胺基转移酶的多肽结合位点的模型,该酶催化GPI修饰。容纳四个残基omega-1 ... omega + 2的活性部位裂口的体积似乎类似于540埃(3)。 [参考:31]

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