关键词: 酸性木聚糖酶；双拷贝菌株；毕赤酵母；体外法

Abstract:

In this study, engineering Pichia pastoris containing double copies of Aspergillus sulphureus xylanase gene xynA was constructed in order to earn a high expression level and low production cost. In a 10 L fermentor, double\|copy recombinant strain yielded the enzyme activity of 3 574 U/mL. The recombinant xylanase exhibited optimal activity at 50℃ and pH 2.2~3.4. Residual activity of the raw recombinant xylanase was over 70%, when fermentation broth was pretreated with Na2HPO4\|citric acid buffer of pH 1.7 for 100 min. And the recombinant xylanase exhibited strong resistance to pepsin and trypsin. High level of catalytic activity in low pH and acid resistance suggested that the recombinant xylanase has a prospective application in feed industry as an additive. Then the recombinant enzymes action effect was rapidly evaluated by in vitro simulating swine gastrointestinal environment. The experiment was conducted to determine the optimal supplementation level of recombinant enzyme in wheat\|based diet preliminarily. In this experiment, wheat\|based diet was divided into 4 treats containing 0, 2 000 U/kg, 4 000 U/kg or 6 000 U/kg recombinant enzyme, with 5 repetitions per treat. Then SDS\|Ⅱ monogastric animal bionic digestive system was used to digest experimental diet by imitating gastrointestinal tract environment of swine. Increasing the level of recombinant acidic β\|1, 4\|xylanase in the diet increased the apparent digestibility of gross energy (GE), crude protein (CP) (linear and quadratic effect; P<0.01) and neutral detergent fibre (NDF) (linear and quadratic effect; P<0.05). The optimal supplementation level of recombinant enzyme was determined to be 4 000 U/kg.

Key words: acidic xylanase, double\, copy strain, pichia pastoris, in vitro method