Purification and general properties of pectin methyl esterase from Curvularia inaequalis NRRL 13884 in solid state culture using orange peels as an inducer.

Acta microbiologica Polonica Pub Date : 2002-01-01
A F Afifi, E M Fawzi, M A Foaad
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Abstract

Pectin methyl esterase (PME) [E.C.3. 1.1.11] production by Curvularia inaequalis (Shear) Boedijn NRRL 13884 was investigated using solid-state culture. The highest level of extracellular pectin methyl esterase was detected with orange peels as an inducing substrate and as a sole carbon source. The enzyme was partially purified using Sephadex G-100 and DEAE-Cellulose column chromatography. It was purified about 40 fold with optimum activity at pH 4.4 and 45 degrees C. The enzyme was activated by Co++, Mg++, Na+, whereas it was slightly activated in the presence of Cu++, K+, Mn++, Zn++. On the other hand Ag++, Ca++ and Hg++ inhibited the activity of the enzyme. The Km was calculated to be 0.52 mM.

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以柑桔皮为诱导剂的曲曲霉(Curvularia inaequalis NRRL 13884)果胶甲基酯酶的固体培养纯化及一般性质研究。
果胶甲基酯酶(PME) [ec .3]。[1.1.11]利用固态培养技术研究了曲霉(Curvularia inaequalis (Shear) Boedijn NRRL 13884)的产量。以柑桔皮为诱导底物和唯一碳源时,细胞外果胶甲基酯酶含量最高。采用Sephadex G-100和DEAE-Cellulose柱层析对酶进行部分纯化。在pH 4.4和45℃条件下,酶活性达到了40倍左右。酶被Co++、Mg++、Na+激活,而在Cu++、K+、Mn++、Zn++存在下酶活性较弱。Ag++、Ca++和Hg++对酶活性有抑制作用。Km计算为0.52 mM。
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