对大豆加工中间产物进行酶水解、同步糖化和发酵,以生产乙醇并浓缩蛋白质和脂质。

ISRN Microbiology Pub Date : 2012-10-17 Print Date: 2012-01-01 DOI:10.5402/2012/278092
Craig C Long, William Gibbons
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引用次数: 0

摘要

大豆中的碳水化合物通常不受欢迎,因为它们消化率低,而且会 "稀释 "更有价值的成分(蛋白质、脂类)。为了去除这些碳水化合物并提高更有价值成分的滴度,研究人员对乙醇生产进行了调查。在磨碎的大豆 (SB)、豆粕 (SBM)、大豆皮 (SH) 和大豆白片 (WF) 中加入商用酶(Novozyme 纤维素酶、β - 葡萄糖苷酶和果胶酶),固体负荷率为 10%,以量化水解葡聚糖。糖化使葡聚糖分别减少 28%、45%、76% 和 80%(SBM、SB、SH、WF)。使用酿酒酵母(Saccharomyces cerevisiae NRRL Y-2034 和 Scheffersomyces stipitis NRRL Y-7124)在 5%、10%、15% 和 20% 固形物添加量下同时进行糖化和发酵(SSF)试验,在 SSF 10% 固形物添加量和糖化试验中分析蛋白质、纤维和脂质。在 SB、SBM 和 WF 上,在所有固体负荷率下,S. cerevisiae 和 S. stipitis 分别产生了 ~3-12.5 克/升乙醇和 ~2.5-8.6 克/升乙醇。SH 可使 S. cerevisiae(~9-23 克/升)和 S. stipitis(~9.5-14.5 克/升)的乙醇滴度更高。蛋白质浓度在 SB、SBM 和 WF 中降低了 2.5-10%,但在 SH 中增加了 53-55%。SB 的油脂浓度增加了约 50%;其他物种的油脂浓度增加了约 500%-1300%。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Enzymatic hydrolysis and simultaneous saccharification and fermentation of soybean processing intermediates for the production of ethanol and concentration of protein and lipids.

Enzymatic hydrolysis and simultaneous saccharification and fermentation of soybean processing intermediates for the production of ethanol and concentration of protein and lipids.

Enzymatic hydrolysis and simultaneous saccharification and fermentation of soybean processing intermediates for the production of ethanol and concentration of protein and lipids.

Enzymatic hydrolysis and simultaneous saccharification and fermentation of soybean processing intermediates for the production of ethanol and concentration of protein and lipids.

Carbohydrates in soybeans are generally undesirable due to their low digestibility and because they "dilute" more valuable components (proteins, lipids). To remove these carbohydrates and raise the titer of more valuable components, ethanol production was investigated. Commercial enzymes (Novozyme cellulase, β -glucosidase, and pectinase) were added to ground soybeans (SB), soybean meal (SBM), soybean hulls (SH), and soybean white flakes (WF) at a 10% solids loading rate to quantify hydrolyzed glucan. Saccharification resulted in glucan reductions of 28%, 45%, 76%, and 80% (SBM, SB, SH, WF, resp.). Simultaneous saccharification and fermentation (SSF) trials were conducted at 5%, 10%, 15%, and 20% solids loading with Saccharomyces cerevisiae NRRL Y-2034 and Scheffersomyces stipitis NRRL Y-7124, with protein, fiber, and lipids analyzed at SSF 10% solids and saccharification trials. S. cerevisiae and S. stipitis produced ~3-12.5 g/L ethanol and ~2.5-8.6 g/L ethanol, respectively, on SB, SBM, and WF over all solid loading rates. SH resulted in higher ethanol titers for both S. cerevisiae (~9-23 g/L) and S. stipitis (~9.5-14.5 g/L). Protein concentrations decreased by 2.5-10% for the SB, SBM, and WF, but increased by 53%-55% in SH. Oil concentrations increased by ~50% for SB; by ~500%-1300% for the others.

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