Heterologous Expression of Extracellular Proteinase pAsPs of Aspergillus pseudotamarii in Komagataella phaffii
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Published:2022-11-30
Issue:23
Volume:23
Page:15035
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ISSN:1422-0067
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Container-title:International Journal of Molecular Sciences
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language:en
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Short-container-title:IJMS
Author:
Zadorozhny Andrey Valentinovich, Voskoboev Mikhail Evgenyevich, Bochkov Denis Vladimirovich, Rozanov Alexei Sergeyevich, Shedko Elizaveta DmitrievnaORCID, Mescheryakova Irina Anatolyevna, Blinov Alexander Gennadyevich, Korzhuk Anton Vladimirovich, Shlyakhtun Valeria Nikolayevna, Bogacheva Natalia Vladimirovna, Antonov Egor Vladimirovich, Bannikova Svetlana Valerevna, Goryachkovskaya Tatiana Nikolayevna, Peltek Sergey Evgenyevich
Abstract
Neutral protease pAsPs gene was obtained by sequence optimization of NpI protease from Aspergillus pseudotamarii. pAsPs was for the first time integrated in the genome of yeast strain Komagataella phaffii T07, and then produced in a 5 L bioreactor with an enzyme yield of 150,800 U/mL of culture liquid towards casein. The specific activity of the pAsPs was 7,657,000 U/mg toward casein, 2320 U/mg toward hemoglobin, and 25,344 U/mg toward azocasein per 1 mg of the protein. The enzyme was found to be inhibited by Cu2+. Optimal activity pH was shown in the range of pH 6.5–8.0, and optimal temperature—50–60 °C. The molecular mass of the recombinant protease pAsPs was shown to be 67.5 kDa. Mass-spectrometric analysis confirmed the identity of the amino acid sequence of the obtained pAsPs preparation with the predicted sequence, with 17% coverage and protein score 288. Thus, the novel neutral protease pAsPs is a promising candidate for large-scale use in manufacturing, including the food industry.
Funder
Ministry of Science and Higher Education of the Russian Federation
Subject
Inorganic Chemistry,Organic Chemistry,Physical and Theoretical Chemistry,Computer Science Applications,Spectroscopy,Molecular Biology,General Medicine,Catalysis
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