(丝氨酸-磷脂酰)-尿扩张素的合成、纯化及生物活性研究。

H Mostafavi, K Adermann, S Austermann, M Raida, M Meyer, W G Forssmann
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引用次数: 0

摘要

基于全局磷酸化的方法,选择性合成(ser10 -磷脂酰)-尿扩张素(phosphourodilatin),它包含32个氨基酸残基和一个二硫环。利用fmoc -化学方法在聚乙二醇-聚苯乙烯载体上逐步组装该肽。在1小时内,用过量的二叔丁基- n, n-二乙基磷酸酰胺进行磷酸化,然后用过氧化叔丁基氧化得到受保护的磷酸肽。用碘滴定法对单乙酰氨基甲基保护的粗肽进行了无副反应的二硫桥的引入。在合成途径中,与侧链无保护的fmoc -丝氨酸的酰化和磷酸化令人满意地产生了预期的中间体。在一些磷酸化实验中,观察到一种与h -膦酸盐相应质量降低的副产物。以磷酸扩张素的合成为例,这种无法用HPLC分离的副产物,以及复杂的氨基酸序列,使得合成一个大的磷酸肽比合成短的磷酸肽更加复杂,短的磷酸肽不含氧化敏感的氨基酸、复杂的序列或额外的结构元素,如二硫环。在两种测定系统中比较了尿舒张素与非磷酸化尿舒张素的生物活性。两种多肽均对主动脉平滑肌条有血管松弛作用,并诱导RFL-6细胞产生cgmp,且剂量依赖性增强。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Synthesis, purification and biological activity of (Ser10-phosphatidyl)-urodilatin (phosphourodilatin).

Based on the global phosphorylation approach, a selective synthesis of (Ser10-phosphatidyl)-urodilatin (phosphourodilatin), which contains 32 amino acid residues and a disulfide loop is described. The peptide was assembled stepwise on a polyethyleneglycol-polystyrene support using Fmoc-chemistry. The phosphorylation was performed on-resin by phosphitylation with a large excess of di-tert-butyl-N,N-diethylphosphoramidite within 1 hour, followed by oxidation with tert-butylhydroperoxide to the protected phosphopeptide. After cleavage and deprotection the disulfide bridge was introduced without side reactions by iodine titration of the mono-acetamidomethyl protected crude peptide. During the synthetic pathway, the acylation with side chain-unprotected Fmoc-serine and the phosphitylation satisfactorily yielded the expected intermediates. In some phosphorylation experiments a by-product having a reduced mass corresponding to the H-phosphonate was observed. Illustrated with the synthesis of phosphourodilatin, this type of by-product, which could not be separated by HPLC, and the difficult amino acid sequence make the synthesis of a large phosphopeptide a more delicate task than the synthesis of short phosphopeptides, which do not contain oxidation-sensitive amino acids, difficult sequences or additional structural elements such as disulfide loops. The biological activity of phosphourodilatin was compared with non-phosphorylated urodilatin in two assay systems. Both peptides revealed a vasorelaxant effect on aortic smooth muscle strips and induced a cGMP-generation in RFL-6 cells with increasing dose dependency.

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