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使用固定在果胶凝胶中的糖化酶和酵母从淀粉中连续生产乙醇。

Continuous production of ethanol from starch using glucoamylase and yeast co-immobilized in pectin gel.

作者信息

Giordano Raquel L C, Trovati Joubert, Schmidell Willibaldo

机构信息

Chemical Engineering Department, Universidade Federal de São Carlos, Washington Luiz, Monjolinho, São Carlos, Brazil.

出版信息

Appl Biochem Biotechnol. 2008 Mar;147(1-3):47-61. doi: 10.1007/s12010-007-8067-1. Epub 2007 Nov 8.

DOI:10.1007/s12010-007-8067-1
PMID:18401752
Abstract

This work presents a continuous simultaneous saccharification and fermentation (SSF) process to produce ethanol from starch using glucoamylase and Saccharomyces cerevisiae co-immobilized in pectin gel. The enzyme was immobilized on macroporous silica, after silanization and activation of the support with glutaraldehyde. The silica-enzyme derivative was co-immobilized with yeast in pectin gel. This biocatalyst was used to produce ethanol from liquefied manioc root flour syrup, in three fixed bed reactors. The initial reactor yeast load was 0.05 g wet yeast/ml of reactor (0.1 g wet yeast/g gel), used in all SSF experiments. The enzyme concentration in the reactor was defined by running SSF batch assays, using different amount of silica-enzyme derivative, co-immobilized with yeast in pectin gel. The chosen reactor enzyme concentration, 3.77 U/ml, allowed fermentation to be the rate-limiting step in the batch experiment. In this condition, using initial substrate concentration of 166.0 g/l of total reducing sugars (TRS), 1 ml gel/1 ml of medium, ethanol productivity of 8.3 g/l/h was achieved, for total conversion of starch to ethanol and 91% of the theoretical yield. In the continuous runs, feeding 163.0 g/l of TRS and using the same enzyme and yeast concentrations used in the batch run, ethanol productivity was 5.9 g ethanol/l/h, with 97% of substrate conversion and 81% of the ethanol theoretical yield. Diffusion effects in the extra-biocatalyst film seemed to be reduced when operating at superficial velocities above 3.7 x 10(-4) cm/s.

摘要

本研究提出了一种连续同步糖化发酵(SSF)工艺,该工艺使用固定在果胶凝胶中的糖化酶和酿酒酵母从淀粉生产乙醇。酶在经硅烷化并用戊二醛活化载体后固定在大孔二氧化硅上。二氧化硅 - 酶衍生物与酵母共同固定在果胶凝胶中。这种生物催化剂用于在三个固定床反应器中从液化木薯根粉糖浆生产乙醇。在所有SSF实验中,初始反应器酵母负载量为0.05 g湿酵母/ ml反应器(0.1 g湿酵母/ g凝胶)。通过进行SSF分批试验来确定反应器中的酶浓度,试验中使用不同量的与酵母共同固定在果胶凝胶中的二氧化硅 - 酶衍生物。所选的反应器酶浓度为3.77 U / ml,使得发酵成为分批实验中的限速步骤。在此条件下,使用初始底物浓度为166.0 g / l的总还原糖(TRS)、1 ml凝胶/ 1 ml培养基,实现了8.3 g / l / h的乙醇生产率,淀粉完全转化为乙醇,达到理论产率的91%。在连续运行中,进料163.0 g / l的TRS并使用与分批运行相同的酶和酵母浓度,乙醇生产率为5.9 g乙醇/ l / h,底物转化率为97%,乙醇理论产率为81%。当在高于3.7×10(-4)cm / s的表观速度下运行时,生物催化剂外膜中的扩散效应似乎有所降低。

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