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乳酸杆菌LBL-4氨肽酶对蛋白质水解物的脱苦作用

Debittering of Protein Hydrolysates by Lactobacillus LBL-4 Aminopeptidase.

作者信息

Tchorbanov Bozhidar, Marinova Margarita, Grozeva Lydia

机构信息

Institute of Organic Chemistry with Centre of Phytochemistry, Bulgarian Academy of Sciences, Acad. G. Bonchev Str. 9, 1113 Sofia, Bulgaria.

出版信息

Enzyme Res. 2011;2011:538676. doi: 10.4061/2011/538676. Epub 2011 Aug 24.

Abstract

Yoghurt strain Lactobacillus LBL-4 cultivated for 8-10 h at pH ~6.0 was investigated as a considerable food-grade source of intracellular aminopeptidase. Cell-free extract manifesting >200 AP U/l was obtained from cells harvested from 1 L culture media. Subtilisin-induced hydrolysates of casein, soybean isolate, and Scenedesmus cell protein with degree of hydrolysis 20-22% incubated at 45°C for 10 h by 10 AP U/g peptides caused an enlarging of DH up to 40-42%, 46-48%, and 38-40% respectively. The DH increased rapidly during the first 4 h, but gel chromatography studies on BioGel P-2 showed significant changes occurred during 4-10 h of enzyme action when the DH increased gradually. After the digestion, the remained AP activity can be recovered by ultrafiltration (yield 40-50%). Scenedesmus protein hydrolysate with DH 20% was inoculated by Lactobacillus LBL-4 cells, and after 72 h cultivation the DH reached 32%. The protein hydrolysates (DH above 40%) obtained from casein and soybean isolate (high Q value) demonstrated a negligible bitterness while Scenedesmus protein hydrolysates (low Q value) after both treatments were free of bitterness.

摘要

研究了在pH值约为6.0的条件下培养8 - 10小时的酸奶菌株乳酸杆菌LBL - 4,它是细胞内氨肽酶的重要食品级来源。从1升培养基收获的细胞中获得了细胞游离提取物,其氨肽酶活性大于200 AP U/l。用枯草杆菌蛋白酶诱导酪蛋白、大豆分离蛋白和栅藻细胞蛋白水解,水解度为20 - 22%,在45℃下用10 AP U/g肽孵育10小时,分别使水解度提高到40 - 42%、46 - 48%和38 - 40%。水解度在最初4小时内迅速增加,但对BioGel P - 2进行凝胶色谱研究表明,在酶作用的4 - 10小时内发生了显著变化,此时水解度逐渐增加。消化后,剩余的氨肽酶活性可通过超滤回收(回收率40 - 50%)。用乳酸杆菌LBL - 4细胞接种水解度为20%的栅藻蛋白水解物,培养72小时后,水解度达到32%。从酪蛋白和大豆分离蛋白(高Q值)获得的蛋白水解物(水解度高于40%)苦味可忽略不计,而两种处理后的栅藻蛋白水解物(低Q值)均无苦味。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c399/3162980/40ee477815c4/ER2011-538676.001.jpg

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