Institute of Biotechnology and Genetic Engineering, Chulalongkorn University, Bangkok, Thailand.
Prep Biochem Biotechnol. 2011;41(2):138-53. doi: 10.1080/10826068.2011.547347.
The objective of this study was to investigate the activity of a protein identified as cysteine protease, purified from Zingiber ottensii Valeton rhizomes, in terms of antiproliferation against fungi, bacteria, and human malignant cell lines. By means of buffer extraction followed by (NH(4))(2)SO(4) precipitation and ion-exchange chromatography, the obtained dominant protein (designated F50) was submitted to non-denaturing and reducing sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), where a single band and three bands were revealed from eletrophoretic patterns, respectively. It could be concluded at this point that the F50 was potentially a heterotrimer or heterodimer composed of either two small (∼13.8 and ∼15.2 kD) subunits or these two together with a larger (∼32.5 kD) one. In-gel digestion was carried out for the most intense band from reducing SDS-PAGE, and to the resulting material was applied liquid chromatography (LC)-mass spectroscopy (MS)/MS. The main F50 subunit was found to contain fragments with 100% similarity to zingipain-1, a cysteine protease first discovered in Zingiber officinale. The activity corresponding to the identified data, cysteine protease, was then confirmed in the F50 by azocasein assay and a positive result was obtained. The F50 then was further investigated for antiproliferation against three plant pathogenic fungi species by disk diffusion test, four bacterial species by direct exposure in liquid culture and dish diffusion tests, and five human malignant cell lines by tissue culture assay. It was found that a dose of 23.6 µg F50/0.3 cm(2) of paper disk exhibited the best inhibitory effect against Collectotrichum cassiicola, while lesser effects were found in Exserohilum turicicum and Fusarium oxysporum, respectively. No inhibitory effect against bacterial proliferation was detected in all studied bacterial strains. However, relatively strong antiproliferative effects were found against five human cell lines, with IC50 values ranging from 1.13 µg/mL (hepatoma cancer; HEP-G2) to 5.37 µg/mL (colon cancer; SW620). By periodic acid-Schiff's staining and phenol-sulfuric acid assay, the F50 was determined as a glycoprotein containing 26.30 ± 1.01% (by weight) of carbohydrate. Thus, a new glycoprotein with protease activity was successfully identified in Zingiber ottensii rhizome. The glycoprotein also contained antiproliferative activity against some plant pathogenic fungi and human cancer cell lines.
本研究旨在探讨从姜黄根茎中分离出的一种被鉴定为半胱氨酸蛋白酶的蛋白质的活性,以评估其对真菌、细菌和人类恶性细胞系的抗增殖作用。通过缓冲液提取,随后进行(NH4)2SO4沉淀和离子交换层析,得到的主要蛋白质(命名为 F50)进行非变性和还原型十二烷基硫酸钠聚丙烯酰胺凝胶电泳(SDS-PAGE),电泳图谱分别显示出一条单带和三条带。由此可以推断,F50 可能是由两个小(约 13.8 和 15.2kD)亚基或这两个亚基与一个较大(约 32.5kD)亚基组成的异三聚体或异二聚体。对还原 SDS-PAGE 中最强烈的条带进行胶内消化,然后对所得物质进行液相色谱(LC)-质谱(MS)/MS 分析。主要的 F50 亚基含有与姜黄蛋白酶-1(Zingipain-1)完全相同的片段,姜黄蛋白酶-1 是首次在姜黄中发现的一种半胱氨酸蛋白酶。通过偶氮酪蛋白测定法和阳性结果,进一步证实了鉴定数据中 F50 的半胱氨酸蛋白酶活性。然后,通过圆盘扩散试验研究 F50 对三种植物病原真菌的抗增殖作用,通过液体培养和盘扩散试验研究四种细菌对 F50 的直接暴露,通过组织培养试验研究 F50 对五种人类恶性细胞系的抗增殖作用。结果发现,剂量为 23.6μg F50/0.3cm2 的纸碟对胶孢炭疽菌表现出最佳的抑制作用,而对突脐蠕孢菌和尖孢镰刀菌的抑制作用较小。在所有研究的细菌菌株中均未检测到对细菌增殖的抑制作用。然而,对五种人类细胞系表现出相对较强的抗增殖作用,IC50 值范围从 1.13μg/mL(肝癌;HEP-G2)到 5.37μg/mL(结肠癌;SW620)。通过过碘酸希夫染色和苯酚-硫酸法测定,F50 被确定为一种含有 26.30±1.01%(按重量计)碳水化合物的糖蛋白。因此,成功地从姜黄根茎中鉴定出一种具有蛋白酶活性的新糖蛋白。该糖蛋白还含有对一些植物病原真菌和人类癌细胞系的抗增殖活性。
