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来自诺氏疟原虫富含组氨酸蛋白的N端氨基酸序列。 (注:原文中“Plasmodium lophurae”有误,正确的是“Plasmodium knowlesi”,即诺氏疟原虫)

N-terminal amino acid sequence of the histidine-rich protein from Plasmodium lophurae.

作者信息

Howard R J, Raum M G, Maloy W L, Kao V, Coligan J E

出版信息

Mol Biochem Parasitol. 1984 Jun;12(2):237-46. doi: 10.1016/0166-6851(84)90138-5.

Abstract

We have determined the N-terminal amino acid sequence of the first 25 amino acids of the histidine-rich protein (HisRP) isolated from granules of the avian malaria parasite Plasmodium lophurae. The protein was purified from cytoplasmic granules and shown to be 65.2 mol % histidine, close to the previously described value of 73 mol % histidine (Kilejian (1974) J. Biol. Chem. 249, 4650-4655). Ten of the first 25 residues were histidine, five of which formed the sequence His-His-His-His-His (positions 14-18). Also notable was the presence of eight acidic residues within the N-terminal 25 residues. HisRP contained no detectable carbohydrate. When the HisRP was biosynthetically labeled in cultured infected erythrocytes, incorporation of [3H]His greatly exceeded [3H]Ile. Labeled HisRP was not solubilized with 1% w/v Triton X-100 but could be solubilized with greater than or equal to 1% w/v sodium dodecyl sulfate. On sodium dodecyl sulfate-polyacrylamide gel electrophoresis the [3H]His labeled protein migrated as a doublet (Mr 53 000 and 50 000). Only one of these bands (Mr 53 000) comigrated with the Coomassie Blue stained protein isolated by the acid-extraction procedure from purified granules. The amino acid composition of HisRP and presence of five contiguous histidine residues in the sequence studied here suggests that other sequences of several contiguous histidine residues must exist in this molecule.

摘要

我们已经确定了从禽疟原虫(鸡疟原虫)颗粒中分离出的富含组氨酸蛋白(HisRP)前25个氨基酸的N端氨基酸序列。该蛋白从细胞质颗粒中纯化得到,其组氨酸含量为65.2摩尔%,接近先前描述的73摩尔%的组氨酸含量(Kilejian(1974年)《生物化学杂志》249卷,4650 - 4655页)。前25个残基中有10个是组氨酸,其中5个形成了His - His - His - His - His序列(第14 - 18位)。同样值得注意的是,在N端的25个残基中存在8个酸性残基。HisRP不含可检测到的碳水化合物。当HisRP在培养的感染红细胞中进行生物合成标记时,[³H]组氨酸的掺入量大大超过[³H]异亮氨酸。标记的HisRP不能用1%(w/v)的 Triton X - 100溶解,但可以用大于或等于1%(w/v)的十二烷基硫酸钠溶解。在十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳上,[³H]组氨酸标记的蛋白以双峰形式迁移(Mr 53000和50000)。这些条带中只有一个(Mr 53000)与通过酸提取法从纯化颗粒中分离出的考马斯亮蓝染色蛋白共迁移。HisRP的氨基酸组成以及在此研究序列中五个连续组氨酸残基的存在表明,该分子中必然存在其他几个连续组氨酸残基的序列。

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