氮离子入法筛选ε-聚赖氨酸高产菌株

研究氮离子注入法诱变选育ε-聚赖氨酸高产菌株。本文从土壤筛选的菌株TS02出发,通过注入不同剂量30keV氮离子,辅以抗性平板法结合抑菌圈法,筛选出了一株ε-聚赖氨酸高产白色链霉菌(Streptomyces albulus)GC11。经多次传代实验结果表明GC11稳定性良好。摇瓶发酵培养24h,GC11抑菌圈直径为23.20mm,比TS02提高了1.32倍;5L自控发酵罐发酵培养72h,GC11ε-PL产量为4.21g/L,比TS02提高了1.30倍,达到了提高ε-聚赖氨酸产量的目的。

高产辅酶Q_(10)类球红细菌的化学诱变筛选及其发酵培养基优化

利用菌株对(维生素K_3+叠氮化钠+对羟基苯甲酸)的复合抗性作为筛选标记,对产辅酶Q_(10)的类球红细菌(Rhodobacter sphaeroides)使用亚硝基胍进行化学诱变,筛选高产菌株并采用响应面法优化其发酵培养基。结果表明,经诱变选育得到一株遗传稳定的辅酶Q_(10)高产菌株R.sp3-7,其最佳发酵培养基组成为:葡萄糖31.7 g/L,玉米浆干粉5.6 g/L,(NH_4)_2SO_45.3 g/L、谷氨酸钠3.0 g/L、NaCl3.0 g/L、MgSO_4·7H_2O 12.5 g/L、KH_2PO_43.0 g/L、CaCO_32.0 g/L、辅液1 m L/L。在此培养条件下,诱变菌株R.sp3-7的辅酶Q_(10)产量达(93.63±0.59)mg/L,与出发菌株相比提高了116.8%。

紫外和He-Ne激光复合诱变获得高产γ-聚谷氨酸产生菌的研究

以地衣芽孢杆菌(Bacillus licheniformis)BCPG006为出发菌株,通过紫外线和He-Ne激光复合诱变处理,后将诱变菌悬液涂布到抗性平板,选育出一株高产γ-聚谷氨酸的突变株BCPG078,经过摇瓶发酵,培养温度37℃、初始pH7、摇床转速220r/min、培养周期72h,测得γ-聚谷氨酸的产量为16g/L,为出发菌γ-聚谷氨酸的产量(6g/L)的2.67倍。传代实验证明,该突变株遗传性能稳定。说明紫外线和He-Ne激光复合诱变是γ-聚谷氨酸产生菌地衣芽孢杆菌有效的选育方法。

产ε-聚赖氨酸白色链霉菌复合诱变选育研究

白色链霉菌(Streptomyces albulus)出发菌株采用紫外诱变和硫酸二乙酯(DES)化学诱变进行复合诱变处理,处理液接种于甘氨酸和多聚赖氨酸抗性平板选育。通过优化甘氨酸和多聚赖氨酸剂量、紫外照射剂量和化学诱变剂DES剂量等诱变条件,并对诱变后的菌株进行初筛和复筛,最后得到一株较高产ε-多聚赖氨酸的菌株,ε-聚赖氨酸的产量达到0.73g/L的较高水平,是出发菌株的2.2倍。经5次传代发酵表明该菌株稳定。

ε-聚赖氨酸产生菌的复合诱变筛选及其发酵培养基优化

以白色链霉菌FQ-9为出发菌株,首次利用(甘氨酸+L-赖氨酸+磺胺胍)复合抗性,进行"紫外-氯化锂"复合诱变,筛选出一株ε-PL产量达(0.668±0.0045)g/L的突变菌株FQC-23,产量提高了15.37%,且其遗传性稳定。然后在单因素实验的基础上,应用响应面分析方法,对其发酵培养基进行优化,最终确定最佳培养基为(g/L):葡萄糖46.1、酵母粉13.0、(NH4)2SO45.9、Mg SO4·7H2O 0.5、K2HPO40.8、KH2PO41.36、Fe SO4·7H2O 0.03、Zn SO4·7H2O 0.04,在此条件下,FQC-23的ε-PL产量达(1.090±0.0041)g/L,比出发菌株的产量提高了87.56%。

Influence of superplasticizers on the early-age crack resistance of concrete

In order to improve the early-age cracking resistance of concrete, different types of superplasticizers are used. Two types of polycarboxlic salt/acid superplasticizers and one retarding naphthalene superplasticizer are selected to investigate the influence of superplasticizers on the early-age cracking resistance of the concrete by using the slab test and the temperature-stress test. The results show that the polycarboxlic salt/acid superplasticizer cannot always improve the cracking resistance capacity of the concrete compared with the naphthalene superplasticizer, which is related to the chemical structure of the polycarboxlic salt/acid superplasticizer. High plastic tensile strength and dynamic elastic modulus at the early stage are beneficial to avoid cracking, and low hydration heat is also helpful. The evolutions of the drying shrilakage stress and the hydration heat temperature stress varying with time can be comprehensively evaluated by means of the slab test and the temperature stress test.

L-精氨酸高产菌株的亚硝基胍诱变选育和种子培养基的优化研究

为了筛选L-精氨酸的高产菌株,采用亚硝基胍对出发菌株ATCC14067(Brevibacterium flavum)进行诱变,结合抗精氨酸结构类似物D-精氨酸,S-甲基半胱氨酸平板抗性筛选高产菌株,并采用正交试验优化了种子培养基。结果显示,经过1 mg/m L的亚硝基胍诱变处理4 min后,采用14 mg/m L的D-精氨酸抗性平板和8 mg/m L的S-甲基半胱氨酸抗性平板筛选获得精氨酸高产菌株,由于解除精氨酸自身的反馈调节,L-精氨酸积累增大,产酸量达37.2 g/L,比野生菌株提高了128.2%,得到的高产菌株遗传性状稳定。通过对种子培养基进行正交试验优化,确定最终培养基配方为葡萄糖3.0%,玉米浆2.0%,硫酸铵2.0%,KH2PO40.10%,Mg SO4·7H2O 0.05%,尿素0.15%,在此发酵条件下,L-精氨酸产量达37.8 g/L。

Accurate assessment of antibiotic susceptibility and screening resistant strains of a bacterial population by linear gradient plate

The dynamics of a bacterial population exposed to the minimum inhibitory concentration （MIC） of an antibiotic is an important issue in pharmacological research. Therefore, a novel antibiotic susceptibility test is urgently needed that can both precisely determine the MIC and accurately select antibiotic-resistant strains from clinical bacterial populations. For this purpose, we developed a method based on Fick＇s laws of diffusion using agar plates containing a linear gradient of antibiotic. The gradient plate contained two layers. The bottom layer consisted of 15 mL agar containing the appropriate concentration of enrofloxacin and allowed to harden in the form of a wedge with the plate slanted such that the entire bottom was just covered. The upper layer consisted of 15 mL plain nutrient agar added with the plate held in the horizontal position. After allowing vertical diffusion of the drug from the bottom agar layer for 12 h, the enrofloxacin concentration was diluted in proportion to the ratio of the agar layer thicknesses. The uniform linear concentration gradient was verified by measuring the enrofloxacin concentration on the agar surface. When heavy bacterial suspensions were spread on the agar surface and incubated for more than 12 h, only resistant cells were able to form colonies beyond the boundary of confluent growth of susceptible cells. In this way, the true MIC of enrofloxacin was determined. The MICs obtained using this linear gradient plate were consistent with those obtained using conventional antibiotic susceptibility tests. Discrete colonies were then spread onto a gradient plate with higher antibiotic concentrations; the boundary line increased significantly, and gene mutations conferring resistance were identified. This new method enables the rapid identification of resistant strains in the bacterial population. Use of the linear gradient plate can easily identify the precise MIC and reveal the dynamic differentiation of bacteria near the MIC. This method allows the study of genetic and physiological characteristics of individual strains, and may be useful for early warning of antibiotic resistance that may occur after use of certain antirnicrobial agents, and guide clinical treatment.