Extraction of collagenolytic proteases from Aspergillus heteromorphus URM 0269 in an aqueous two-phase system for application in collagen hydrolysis

被引:0
|
作者
da Costa, Beatriz de Aquino Marques [1 ]
de Araujo, Ana Claudia Vaz [2 ]
Fernandes, Ligia Maria Goncalves [1 ]
Porto, Ana Lucia Figueiredo [1 ]
Oliveira, Vagne de Melo [3 ]
Porto, Tatiana Souza [1 ]
机构
[1] Rural Fed Univ Pernambuco, Dept Anim Morphol & Physiol, Recife, Brazil
[2] Univ Fed Rural Pernambuco, Acad Unit Cabo de Santo Agostinho, BR-54518430 Recife, PE, Brazil
[3] Univ Fed Acre, Ctr Hlth & Sports Sci, Rio Branco, Brazil
来源
关键词
Fish waste; enzyme partitioning; collagen extraction; ACID-SOLUBLE COLLAGEN; BIOCHEMICAL-CHARACTERIZATION; PENICILLIUM-AURANTIOGRISEUM; ALKALINE PROTEASE; PURIFICATION; SKIN; SCAFFOLD; BONE;
D O I
10.1080/10826068.2023.2263870
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Collagenolytic proteases produced by Aspergillus heteromorphus URM0269 were extracted using a PEG/sulfate aqueous two-phase system (ATPS). A 2(3) factorial design was performed to analyze the independent variables: PEG molar mass (M-PEG), PEG concentration (C-PEG), and sulfate concentration (C-sulf). The extracted proteases were also evaluated for their optimum pH and stability at different pH levels (4.0 - 11.0) after 20 h of incubation. Collagen was extracted from mutton snapper (Lutjanus analis) skin using acetic acid (0.5 mol L-1). The enzyme was preferentially partitioned to the PEG-rich phase (K > 1), whose highest purification factor and recovery (PF = 6.256 and Y = 404.432%) were obtained under specific conditions: M-PEG 8000 g.mol(-1), C-PEG 30%, C-sulf 10%. The ATPS extraction provided an enzymatic activity range of pH 7.0 - 11.0, exhibiting greater stability compared to the crude extract. Approximately 80% of protease activity was maintained after 20 hours of incubation at all analyzed pH levels, except pH 11.0. Collagen extraction from L. analis skin yielded 8.056%, and both crude extract samples and ATPS-derived samples successfully hydrolyzed the extracted collagen, reaching peak hydrolysis after 36 hours of treatment. These findings demonstrate the feasibility of extracting highly purified and active proteases capable of hydrolyzing L. analis collagen.
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收藏
页码:647 / 659
页数:13
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