State Key Laboratory of Food Science and Technology, The Key Laboratory of Industrial Biotechnology of Ministry of Education, School of Biotechnology, Jiangnan University, 1800 Lihu Ave, Wuxi 214122, Jiangsu, China.
J Ind Microbiol Biotechnol. 2013 Aug;40(8):855-64. doi: 10.1007/s10295-013-1284-4. Epub 2013 May 18.
A novel endoprotease Endo-Pro-Aspergillus niger (endoprotease EPR) was first successfully expressed at high level in the methylotrophic yeast Pichia pastoris and the purification procedure was established. The endoprotease EPR is 95 % identity with proline specific endopeptidase from A. niger CBS513.88 (EMBL; AX458699), while sharing low identity with those from other microorganisms. The purified endoprotease EPR was a monomer of 60 kDa. Furthermore, the peptide mass fingerprinting (PMF) analysis confirmed that the purified protein was an endoprotease Endo-Pro-Aspergillus niger. A three-dimensional model revealed that the active site of the enzyme was located in Ser(179)-Asp(458)-His(491), based on template 3n2zB with sequence identity of 17.6 %. The optimum pH and temperature of the endoprotease EPR were pH 4-5 and 35 °C, and the stabilities were pH 3-7 and 15-60 °C, respectively. Furthermore, the endoprotease EPR had the ability to digest peptides with the C-terminal of proline as well as alanine, and was also capable of hydrolyzing larger peptides. The properties of the endoprotease EPR made it a highly promising candidate for future application in the field of brewing and food process.
一种新型内切蛋白酶 Endo-Pro-黑曲霉(内切蛋白酶 EPR)首次在甲醇营养酵母毕赤酵母中高水平成功表达,并建立了纯化程序。内切蛋白酶 EPR 与黑曲霉 CBS513.88 的脯氨酸特异性内肽酶(EMBL;AX458699)具有 95%的同一性,而与其他微生物的同一性较低。纯化的内切蛋白酶 EPR 是一个 60 kDa 的单体。此外,肽质量指纹图谱(PMF)分析证实,纯化的蛋白质是一种内切蛋白酶 Endo-Pro-黑曲霉。三维模型显示,根据序列同一性为 17.6%的模板 3n2zB,该酶的活性位点位于 Ser(179)-Asp(458)-His(491)。内切蛋白酶 EPR 的最适 pH 和温度分别为 pH4-5 和 35°C,稳定性分别为 pH3-7 和 15-60°C。此外,内切蛋白酶 EPR 具有消化 C 末端为脯氨酸和丙氨酸的肽的能力,并且还能够水解较大的肽。内切蛋白酶 EPR 的性质使其成为未来在酿造和食品加工领域应用的极具前景的候选酶。
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