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首页> 外文期刊>Applied and Environmental Microbiology >Analysis of xysA, a gene from Streptomyces halstedii JM8 that encodes a 45-kilodalton modular xylanase, Xys1.
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Analysis of xysA, a gene from Streptomyces halstedii JM8 that encodes a 45-kilodalton modular xylanase, Xys1.

机译:分析xysA,这是一种来自Halstedii链霉菌JM8的基因,该基因编码45公斤的模块化木聚糖酶Xys1。

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摘要

The gene xysA from Streptomyces halstedii JM8 encodes a protein of 461 amino acids (Xys1) which is secreted into the culture supernatant as a protein of 45 kDa (Xys1L). Later, this form is proteolytically processed after residue D-362 to produce the protein Xys1S, which conserves the same xylanolytic activity. The cleavage removes a domain of 99 amino acids that shows similarity to bacterial cellulose binding domains and that allows the protein Xys1L to bind to crystalline cellulose (Avicel). Expression of this monocistronic gene is affected by the carbon source present in the culture medium, xylan being the best inducer. By using an anti-Xys1L serum, we have been able to detect xylanases similar in size to Xys1L and Xys1S in most of the different Streptomyces species analyzed, suggesting the ubiquity of these types of xylanases and their processing mechanism.
机译:halstedii链霉菌JM8的xysA基因编码一个461个氨基酸的蛋白质(Xys1),并以45 kDa的蛋白质(Xys1L)的形式分泌到培养上清液中。后来,在残基D-362之后对这种形式进行蛋白水解处理,以产生蛋白Xys1S,该蛋白保留了相同的木聚糖分解活性。该切割去除了99个氨基酸的结构域,该结构域显示与细菌纤维素结合结构域的相似性,并允许蛋白质Xys1L与结晶纤维素(Avicel)结合。该单顺反子基因的表达受培养基中存在的碳源的影响,木聚糖是最好的诱导剂。通过使用抗Xys1L血清,我们已经能够在分析的大多数不同链霉菌种中检测到大小与Xys1L和Xys1S相似的木聚糖酶,表明这些木聚糖酶类型及其加工机理无处不在。

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