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首页> 外文期刊>Applied and Environmental Microbiology >Chitinase-overproducing mutant of Serratia marcescens.
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Chitinase-overproducing mutant of Serratia marcescens.

机译:粘质沙雷氏菌的几丁质酶过量生产突变体。

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Genetic modification of Serratia marcescens QMB1466 was undertaken to isolated mutants which produce increased levels of chitinolytic activity. After mutagenesis with ultraviolet light, ethyl methane sulfonate or N-methyl-N'-nitro-N-nitrosoguanidine, 19,940 colonies were screened for production of enlarged zones of clearing (indicative of chitinase activity) on chitin-containing agar plates. Forty-four chitinase high producers were tested further in shake flask cultures. Mutant IMR-1E1 was isolated which, depending on medium composition, produced two to three times more than the wild type of the other components of the chitinolytic enzyme system--a factor involved in the hydrolysis of crystalline chitin and chitobiase. After induction by chitin, endochitinase and chitobiase activity appeared at similar times for both IMR-1E1 and QMB1466, suggesting possible coordinate control of these enzymes. The results are consistent with IMR-1E1 containing a regulatory mutation which increased production of the components of the chitinolytic enzyme system and/or with IMR-1E1 containing a tandem duplication of the chitinase genes. The high rate of reversion of IMR-1E1 to decreased levels of chitinase production suggests that the overproduction of chitinase by IMR-1E1 is due to a tandem gene duplication.
机译:对分离的突变体进行了粘质沙雷氏菌QMB1466的遗传修饰,产生高水平的几丁质分解活性。在用紫外线,甲烷磺酸乙酯或N-甲基-N'-硝基-N-亚硝基胍诱变后,筛选了19,940个菌落,以在含几丁质的琼脂平板上产生更大的清除区域(指示几丁质酶活性)。在摇瓶培养中进一步测试了44个几丁质酶高产者。分离出的突变体IMR-1E1取决于培养基的组成,其产量是几丁质分解酶系统其他组分的野生型的2至3倍-这是结晶几丁质和几丁质酶水解的一个因素。几丁质诱导后,IMR-1E1和QMB1466的内切几丁质酶和几丁质酶活性在相似的时间出现,表明可能对这些酶进行协调控制。该结果与含有调节突变的IMR-1E1和/或与含有串联几丁质酶基因的IMR-1E1一致,IMR-1E1含有调节突变,其增加了几丁质分解酶系统的成分的产生。 IMR-1E1高度回复到几丁质酶生产水平降低表明,IMR-1E1过几丁质酶的过量生产是由于串联基因重复。

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