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重组甲硫氨酰胰岛素样生长因子-I变体的结合蛋白、放射受体及生物学活性

Binding protein, radioreceptor and biological activities of recombinant methionyl insulin-like growth factor-I variants.

作者信息

Hodgkinson S C, Napier J R, Davis S R, Patel B, Gluckman P D

机构信息

Ruakura Agricultural Centre, Ministry of Agriculture and Fisheries, Hamilton, New Zealand.

出版信息

Mol Cell Endocrinol. 1989 Sep;66(1):37-44. doi: 10.1016/0303-7207(89)90046-4.

Abstract

Reversed-phase chromatography (RPC) was used to resolve two variants of recombinant amino terminal methionyl residue (N-Met) insulin-like growth factor-I (IGF-I) with the same amino acid constitution but different disulphide linkages. Following radioiodination, equilibration with plasma and size exclusion chromatography at neutral pH the major form on RPC (approximate abundance 60%) demonstrated greater than 80% binding to 150 kDa and 40-50 kDa IGF binding proteins. This peptide has the RPC elution characteristics and disulphide assignment (Cys6-Cys48, Cys18-Cys61, Cys47-Cys52) of authentic with mismatched disulphides (Cys6-Cys47, Cys18-Cys61, Cys48-Cys52; N-Met IGF-I peak 1 peptide) demonstrated less than 15% binding under similar conditions. Potency of the peptides was investigated in competitive IGF-I plasma binding protein and L6 myoblast radioreceptor assays. The peak 2 peptide proved equipotent to purified ovine plasma IGF-I in each system but by contrast the peak 1 peptide was 40-fold and 200-fold less potent in the binding protein and radioreceptor assays respectively. Biological potency was examined in a non-competitive assay based on incorporation of [3H]leucine into confluent cultures of L6 myoblasts. In this system the N-Met IGF-I peak 1 peptide proved 15-fold less potent than the peak 2 peptide with correct disulphide linkages. Refolding variants may prove useful in establishing structure/function relationships for IGF-I.

摘要

反相色谱法(RPC)用于分离重组氨基末端甲硫氨酰残基(N-甲硫氨酸)胰岛素样生长因子-I(IGF-I)的两种变体,它们具有相同的氨基酸组成,但二硫键不同。经放射性碘化、与血浆平衡以及在中性pH下进行尺寸排阻色谱后,RPC上的主要形式(丰度约为60%)显示与150 kDa和40 - 50 kDa的IGF结合蛋白的结合率大于80%。该肽具有真实IGF-I的RPC洗脱特征和二硫键分配(Cys6-Cys48、Cys18-Cys61、Cys47-Cys52),而二硫键错配的(Cys6-Cys47、Cys18-Cys61.Cys48-Cys52;N-甲硫氨酸IGF-I峰1肽)在类似条件下显示的结合率小于15%。在竞争性IGF-I血浆结合蛋白和L6成肌细胞放射受体测定中研究了这些肽的效力。峰2肽在每个系统中被证明与纯化的绵羊血浆IGF-I效力相当,但相比之下,峰1肽在结合蛋白和放射受体测定中的效力分别低40倍和200倍。基于将[3H]亮氨酸掺入L6成肌细胞汇合培养物的非竞争性测定中检测了生物效力。在该系统中,具有正确二硫键的N-甲硫氨酸IGF-I峰1肽的效力被证明比峰2肽低15倍。重折叠变体可能有助于建立IGF-I的结构/功能关系。

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