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鸟苷酸环化酶C激活肽鸟苷素和尿鸟苷素的合成、生物活性及异构现象

Synthesis, biological activity and isomerism of guanylate cyclase C-activating peptides guanylin and uroguanylin.

作者信息

Klodt J, Kuhn M, Marx U C, Martin S, Rösch P, Forssmann W G, Adermann K

机构信息

Niedersächsisches Institut für Peptid-Forschung (IPF), Hannover, Germany.

出版信息

J Pept Res. 1997 Sep;50(3):222-30. doi: 10.1111/j.1399-3011.1997.tb01188.x.

DOI:10.1111/j.1399-3011.1997.tb01188.x
PMID:9309586
Abstract

Recently, the peptides guanylin and uroguanylin were identified as endogenous ligands of the membrane-bound guanylate cyclase C (GC-C) that is mainly expressed in the intestinal epithelium. In the present study, bioactive guanylin and uroguanylin have been prepared by solid-phase methodology using Fmoc/HBTU chemistry. The two disulfide bonds with relative 1/3 and 2/4 connectivity have been introduced selectively by air oxidation of thiol groups and iodine treatment of Cys(Acm) residues. Using this strategy, several sequential derivatives were prepared. Temperature-dependent HPLC characterization of the bioactive products revealed that guanylin-related peptides exist as a mixture of two compounds. The isoforms are interconverted within approximately 90 min, which prevents their separate characterization. This effect was not detected for uroguanylin-like peptides. Synthetic peptides were tested for their potential to activate GC-C in cultured human colon carcinoma cells (T84), known to express high levels of GC-C. The results obtained show that both disulfide bonds are necessary for GC-C activation. The presence of the amino-terminally neighboring residues of Cys104 for guanylin and Cys100 for uroguanylin has been found to be essential for GC-C stimulation. Unexpectedly, a hybrid peptide obtained from substitution of the central tripeptide AYA of guanylin by the tripeptide VNV of uroguanylin was not bioactive.

摘要

最近,鸟苷素和尿鸟苷素这两种肽被鉴定为主要在肠上皮细胞中表达的膜结合鸟苷酸环化酶C(GC-C)的内源性配体。在本研究中,已使用Fmoc/HBTU化学方法通过固相法制备了具有生物活性的鸟苷素和尿鸟苷素。通过硫醇基团的空气氧化和半胱氨酸(Acm)残基的碘处理,选择性地引入了具有相对1/3和2/4连接性的两个二硫键。使用该策略,制备了几种序列衍生物。对生物活性产物进行的温度依赖性高效液相色谱表征表明,鸟苷素相关肽以两种化合物的混合物形式存在。这些异构体在大约90分钟内相互转化,这使得它们无法单独表征。尿鸟苷素样肽未检测到这种效应。对合成肽在已知高表达GC-C的培养人结肠癌细胞(T84)中激活GC-C的潜力进行了测试。所得结果表明,两个二硫键对于GC-C激活都是必需的。已发现鸟苷素中半胱氨酸104和尿鸟苷素中半胱氨酸100的氨基末端相邻残基的存在对于GC-C刺激至关重要。出乎意料的是,通过将鸟苷素的中央三肽AYA替换为尿鸟苷素的三肽VNV获得的杂合肽没有生物活性。

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