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Mutation of Candida tropicalis by Irradiation with a He-Ne Laser To Increase Its Ability To Degrade Phenol▿

机译:He-Ne激光辐照诱变热带假丝酵母,提高其降解苯酚的能力▿

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摘要

Candida tropicalis isolated from acclimated activated sludge was used in this study. Cell suspensions with 5 × 107 cells ml−1 were irradiated by using a He-Ne laser. After mutagenesis, the irradiated cell suspension was diluted and plated on yeast extract-peptone-dextrose (YEPD) medium. Plates with approximately 20 individual colonies were selected, and all individual colonies were harvested for phenol biodegradation. The phenol biodegradation stabilities for 70 phenol biodegradation-positive mutants, mutant strains CTM 1 to 70, ranked according to their original phenol biodegradation potentials, were tested continuously during transfers. Finally, mutant strain CTM 2, which degraded 2,600 mg liter−1 phenol within 70.5 h, was obtained on the basis of its capacity and hereditary stability for phenol biodegradation. The phenol hydroxylase gene sequences were cloned in wild and mutant strains. The results showed that four amino acids were mutated by irradiation with a laser. In order to compare the activity of phenol hydroxylase in wild and mutant strains, their genes were expressed in Escherichia coli BL21(DE3) and enzyme activities were spectrophotometrically determined. It was clear that the activity of phenol hydroxylase was promoted after irradiation with a He-Ne laser. In addition, the cell growth and intrinsic phenol biodegradation kinetics of mutant strain CTM 2 in batch cultures were also described by Haldane's kinetic equation with a wide range of initial phenol concentrations from 0 to 2,600 mg liter−1. The specific growth and degradation rates further demonstrated that the CTM 2 mutant strain possessed a higher capacity to resist phenol toxicity than wild C. tropicalis did.
机译:从驯化的活性污泥中分离出的热带假丝酵母用于本研究。使用He-Ne激光照射5×107细胞ml-1的细胞悬液。诱变后,将辐照后的细胞悬浮液稀释并铺在酵母提取物-蛋白pe-葡萄糖(YEPD)培养基上。选择具有大约20个单个菌落的平板,并收获所有单个菌落用于苯酚生物降解。在转移过程中,连续测试了70种苯酚生物降解阳性突变体(根据其原始苯酚生物降解潜能排名的CTM 1至70突变株)的苯酚生物降解稳定性。最后,根据其对苯酚生物降解的能力和遗传稳定性,获得了在70.5小时内降解了2,600 mg升-1苯酚的突变菌株CTM 2。将酚羟化酶基因序列克隆到野生和突变菌株中。结果表明,通过激光照射使四个氨基酸突变。为了比较野生型和突变型菌株中酚羟化酶的活性,它们的基因在大肠杆菌BL21(DE3)中表达,并通过分光光度法测定酶的活性。清楚的是,用He-Ne激光照射后,酚羟化酶的活性得到提高。此外,分批培养的突变菌株CTM 2的细胞生长和固有苯酚生物降解动力学还通过Haldane动力学方程描述,初始苯酚浓度范围从0到2,600 mg升-1。特定的生长和降解速率进一步证明,CTM 2突变株比野生热带假丝酵母具有更高的抗酚毒性能力。

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