广西科学

引用本文：

叶启腾,陈强,李春香.丝兰酶及其提取工艺的研究[J].广西科学,1995,2(4):6-10. [点击复制]
Ye Qiteng,Chen Qiang,Li Chunxiang.Proteinases of Yucca and Their Extraction[J].Guangxi Sciences,1995,2(4):6-10. [点击复制]

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丝兰酶及其提取工艺的研究
叶启腾, 陈强, 李春香
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(广西亚热带作物研究所, 南宁市邕武路 530001)

摘要:

直接干燥丝兰叶表栅状组织获得粗酶。用硫酸铵分级盐析取得酶制剂,它的最适pH值为12。用有机汞作配基的琼脂糖凝胶4B柱分离出酶,聚丙烯酸胺凝胶电泳证明柱分离物为两个蛋白酶组分(YuccainⅠ、YuccainⅡ),簿层等电聚焦电泳证实这两个组分等电点分别为pH值9.77和pH值9.61,SDS电泳两个酶仅看到1条染色带,测得分子量为3万。它们的活性均依赖于巯基。

关键词: 丝兰酶蛋白酶分离纯化性质

DOI：

投稿时间：1995-05-21

基金项目:国家自然科学基金

Proteinases of Yucca and Their Extraction

Ye Qiteng, Chen Qiang, Li Chunxiang

(Guangxi Institute of Subtropical Crop, Yongwu Road, Nanning, Guangxi, 530001)

Abstract:

The crude enzyme was prepared by dehydration from palisade tissue. The enzyme preparation with an optimal pH of 12 was salted out with (NH₄)₂SO₄. Two fractions obtained by chromatography on sepharose 4B column with organic mercury dentate were Yuccains Ⅰ, Ⅱ (proteinases) using electrophoresis in thin polyacrylamide gel. YuccainsⅠ, Ⅱ just showed one strip in SDSPAGE, and their molecular weithts were 30000 and isoelectric points were PH values of 9.77 and 9.61 respectively. Their activities were subject to the SH-.

Key words: Yuccain proteinase extraction purification property

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