高产辅酶Q10结构类似物抗性突变株的选育

以土壤杆菌(Agrobacteriumsp.)TLY-4为出发菌株,采用70%致死剂量的NTG进行诱变处理,通过筛选抗辅酶Q10结构类似物维生素K3突变株,定向选育到了两株辅酶Q10高产突变株,编号为R-122和R-015,其摇瓶发酵72h时的辅酶Q10产量分别为57.3 mg/L和59.9 mg/L,较出发菌株提高了35.7%和41.6%。通过连续传代实验,表明突变株高产辅酶Q10的遗传性状稳定。实验以有机溶剂DMF和吐温-80共同增溶的方法,解决了维生素K3在培养基中易析出的问题,并确定了平板培养基中维生素K3的最小抑菌浓度为0.15 mg/mL。     

辅酶Q10产生菌的抗性筛选及发酵条件优化

以根癌土壤杆菌(Agrobacterium tumefaciens)WSHAT12为出发菌株,通过硫酸二乙酯诱变,获得遗传稳定性好的抗L-乙硫氨酸(Eth)突变株WSH-E01,通过进一步的诱变处理,获得L-乙硫氨酸和维生素K3(VK3)双抗性突变株WSH-V01,以双抗性突变株WSH-V01为出发菌株,再进行诱变处理,获得一株X-gal利用能力提高的突变株WSH-X01,与出发菌株WSHAT12相比,突变株WSH-X01的辅酶Q10产量提高幅度达50.6%,同时,对突变株WSH-E01的发酵条件进行优化。出发菌株WSHAT12、突变株WSH-E01、WSH-V01和WSH-X01在优化后的发酵条件下辅酶Q10产量分别达到23.1mg/L、26.8mg/L、29.5mg/L和34.8mg/L。     

离子束诱变粟酒裂殖酵母产辅酶Q_(10)的初步研究

辅酶Q10(coenzyme Q10,CoQ)对心脏充血性病人有较好的疗效,是临床常用药物之一。实验研究了离子束诱变粟酒裂殖酵母对提高CoQ10的产量的影响与作用。实验筛选出六株突变菌株,研究了突变株生理生化特性。结果表明:突变菌株的CoQ10产量都有不同程度的提高,其中编号为N1菌株产量达6.9344mg/L,是对照菌株的10倍多,最低的N2菌株的产量也是对照菌株的1.3倍。     

离子束诱变粟酒裂殖酵母产辅酶Q10的初步研究

辅酶Q10(coenzyme Q10,CoQ)对心脏充血性病人有较好的疗效,是临床常用药物之一.实验研究了离子束诱变粟酒裂殖酵母对提高CoQ10的产量的影响与作用.实验筛选出六株突变菌株,研究了突变株生理生化特性.结果表明:突变菌株的CoQ10产量都有不同程度的提高,其中编号为N1菌株产量达6.9344 mg/L,是对照菌株的10倍多,最低的N2菌株的产量也是对照菌株的1.3倍.     

ɑ-乙酰乳酸脱羧酶产生菌的微波诱变

为获得ɑ-乙酰乳酸脱羧酶的高产突变株,以产ɑ-ALDC的枯草芽孢杆菌3226-5为出发菌株进行了诱变处理。经过微波(小火)物理诱变得到3株高产正突变株W181、W184、W195,经过多次传代实验,表明W181、W195是稳定的突变株。突变株W195的ɑ-ALDC相对酶活(OD522)由出发菌株的0.35提高到0.617,提高了76%,突变株W181提高了66.9%。     

产L-谷氨酸工程菌株的诱变选育及其发酵效率

以高产L-谷氨酸的谷氨酸棒杆菌GY1为研究对象,采用ARTP进行全局诱变,进一步提高L-谷氨酸的发酵水平。首先,对谷氨酸棒杆菌GY1原生质体的制备及再生条件进行优化,接着,根据致死率选择最佳的ARTP处理时间,然后,采用96微孔板及摇瓶发酵的方式对突变株进行筛选,最后,对获得的优良突变株进行50 L罐发酵验证。结果显示,溶菌酶浓度为10.0 mg/mL,酶解90 min,原生质体形成率和再生率达到最佳。ARTP最佳处理时间为40 s,致死率达到89.6%,经过初筛与摇瓶复筛,获得突变株YAG117,其摇瓶发酵L-谷氨酸含量达16.3 g/L,较出发菌株提高13.9%,且连续传代五代遗传稳定。50 L补料分批发酵条件下,L-谷氨酸产量在36 h最高,达到216.6 g/L,较出发菌株提高12.9%,糖酸转化率达68.87%,比出发菌株提高了10.2%。ARTP处理GY1菌株原生质体,能够有效积累有利突变,提高突变株发酵生产L-谷氨酸的能力,获得的突变株YAG117也显示了较好的工业化应用潜力。     

HNO_2诱变选育链霉菌702菌株

以链霉菌702-20为出发菌株,经HNO2诱变处理,获得高产突变株。实验结果表明:HNO2处理20 m in对菌株的致死率可达83.10%,突变率高达14.13%,经过摇瓶筛选获得高产突变株20-29-148,产链霉素能力达到1.404 mg/mL,比出发菌株提高了37.65%。经传代培养考察,该突变菌株具有良好的遗传稳定性。     

谷胱甘肽高产菌株的选育

以编号为 346的酿酒酵母为出发菌株 ,通过紫外线和_{60Coγ射线诱变处理 ,运用推理育种技术 ,选育到一株抗氯化锌和乙硫氨酸的突变株 0 5Eth40 0 5。该菌株经摇瓶发酵谷胱甘肽产量为 1 65 96mg L ,较出发株提高 350 % ,每克干细胞含谷胱甘肽 1 9 76mg ,较出发株提高 31 8 6 %。菌株经 1 0次传代培养 ,谷胱甘肽产量下降 1 0 7% ,是一株性状较稳定可深入开发研究的优良菌株。}     

α-乙酰乳酸脱羧酶产生菌的微波诱变

为获得α-乙酰乳酸脱羧酶的高产突变株,以产α-ALDC的枯草芽孢杆菌3226—5为出发菌株进行了诱变处理。经过微波（小火）物理诱变得到3株高产正突变株W181、W184、W195,经过多次传代实验,表明W181、W195是稳定的突变株。突变株W195的α-ALDC相对酶活（OD522）由出发菌株的0．35提高到0．617,提高了76％,突变株W181提高了66．9％。     

产脲酶芽胞杆菌的微波诱变育种

巴氏芽胞杆菌是目前微生物诱导碳酸钙沉淀(MICP)方法中应用最为热门的一种细菌。为提高巴氏芽胞杆菌尿素分解以及矿化能力,以巴氏芽胞杆菌YB-B为出发菌株,采用微波诱变育种技术,通过诱变菌株特性筛选及其遗传稳定性检测,成功选育出2株突变菌株YB-3和YB-4。与出发菌株相比,诱变菌株尿素分解能力较原菌株提高1.5倍左右,矿化能力提高114%。诱变菌株具有生长速度快,环境适应性强,矿化能力高等优点,这为MICP更广层次的应用奠定了坚实的基础。     

ENHANCED β-GALACTOSIDASE PRODUCTION OF Aspergillus oryzae MUTATED BY UV AND LiCl

In order to breed a high-yield β-galactosidase-producing strain, Aspergillus oryzae was used as the parent strain and mutagenized with ultraviolet (UV) and UV plus lithium chloride (LiCl), respectively. After being mutagenized by UV, the β-galactosidase activity of mutant UV-15-20 reached 114.08 U/mL, which revealed a 49.22% increase compared with the original strain. A mutant UV-LiCl-38 with high β-galactosidase activity (121.42U/mL) was obtained after compound mutagenesis of UV and LiCl; the β-galactosidase activity of this mutant was 58.82% higher than that of the parent strain. Subculture testing indicated that UV-15-20 and UV-LiCl-38 had good hereditary stability and may be ideal strains for the production of β-galactosidase. Additionally, it was demonstrated that compound mutagenesis with UV and LiCl is an effective mutation method for breeding industrially interesting strains.     

发酵生产辅酶Q10高产菌株的选育

以实验室保存的类球红细菌(Rhodobacter sphaeroides)JDW61为出发菌株,考察了紫外、紫外结合氯化锂和亚硝基胍对菌株产生辅酶Q10能力的诱变效应,并结合辅酶Q10的合成途径设计了快速筛选辅酶Q10高产菌株的模型,获得一株辅酶Q10产量提高的突变株CP222,该菌株摇瓶发酵的辅酶Q10产量为276.14mg·L-1,较出发菌株提高了190%,并且遗传性能稳定。     

用抗性筛选法选育γ—亚麻酸（GLA）高产菌株

以深黄被孢霉（Mortierella isabellina）为出发菌株,经紫外线诱变处理,采用抗性筛选法,直接在梯度平板上挑选取抗脂肪酸脱氢酶抑制物抑芽丹（maleic hydrazide）的菌株进行初筛,然后经摇瓶发酵法测定相关性能指标进行得筛,获得一株生产性能比出发菌株显提高的突变株M80,其菌体收率达25.10g/L、油脂产率达12.35g/L、γ-亚麻酸（GLA）产率达771.88mg/L。     

物化因子结合诱变选育耐温型法夫酵母

以法夫酵母为出发菌株,采用紫外线及甲基磺酸乙酯对其进行诱变育种,筛选出1株最适生长温度比诱变前提高10℃且虾青素产量可达到5．08mg／L的突变菌株,该菌株经多次传代生产性能稳定。     

高产谷胱甘肽的酵母菌选育及其培养条件研究

筛选到一株具有较高GSH产量的酵母菌株S.cerevisiae2165,然后以该菌株为出发菌,采用紫外照射,紫外照射 LiCl联合处理,亚硝基胍（MNNG）等诱变处理,获得一株高产GSH的酿酒酵母优良菌株S.cerevisiaeJN-5-8。该菌株具有稳定的遗传性能,在经过优化的培养条件下培养24h,其GSH产量达到339.1mg/L。比出发菌株提高2.2倍。     

Saccharomyces cerevisiae mutants selected for increased production of Trichoderma reesei cellulases

 Trichoderma reesei endoglucanase I (EGI) was used as a reporter enzyme for screening mutagenized yeast strains for increased ability to produce protein. Sixteen haploid Saccharomyces cerevisiae strains, transformed with a yeast multicopy vector pALK222, containing the EGI cDNA under the ADH1 promoter, produced EGI activity of 10^-5–10^-4 g/l. On the average 93% of the total activity was secreted into the culture medium. Two strains with opposite mating types were mutagenized, and several mutants were isolated possessing up to 45-fold higher EGI activity. The best mutants were remutagenized and a second-generation mutant, strain 2804, with an additional twofold increase in EGI activity was selected. The mutant strain 2804 grew more slowly and reached a lower final cell density than the parental strain. In the selective minimal medium, the 2804 strain produced 40 mg/l immunoreactive EGI protein, but only 2% was active enzyme. In the rich medium the secreted EGI enzyme stayed active, but without selection pressure the EGI production ceased after 2 days of cultivation, when the strain 2804 had produced 10 mg/l of EGI. A sevenfold difference was found between the parental and the 2804 strain in their total EGI production relative to cell density. The difference in favour of the mutant strain was also detected on the mRNA level. The 2804 mutant was found to be more active than the parental strain also in the production of T. reesei cellulases, cellobiohydrolase I, and cellobiohydrolase II. Received: 22 December 1995/Received revision: 26 February 1996/Accepted: 17 March 1996     

果胶酶高产菌种的紫外诱变选育及其培养条件的响应面法优化

以果胶酶产生菌黑曲霉EIM6为出发菌株,初始果胶酶活为14 539 U/mL,经紫外诱变反复处理,摇瓶复筛和遗传稳定性试验,最终获得一株果胶酶高产菌株EIMU2。EIMU2菌株的形态特征发生了明显的改变,相较于原出发菌株EIM6,孢子色泽更黑,孢子团也较出发菌株大,菌丝与孢子上凝结有更多的液珠。复筛后EIMU2酶活为32 161 U/mL,较原出发菌株提高了1.212倍。进一步通过响应面法对EIMU2菌株的液体发酵培养条件进行优化。优化后的培养条件为甜菜渣1.83%,花生饼粉1.69%,(NH_4)_2SO_4 0.5%,K_2HPO_4 0.3%,CaCO_3 0.2%,MgSO_4 0.15%(w/v),接种量6%(v/v),装液量21.36 mL。优化的突变菌株产酶活性进一步提高至98 794.3 U/mL,提高了2.07倍。     

复合诱变选育林肯霉素高产菌株

以林肯链霉菌9502(Streptomyces lincolnensis9502)为出发菌株,进行NTG诱变处理,并用高效的琼脂块培养法对菌株进行筛选,得到产林肯霉素相对效价提高35.4%的变异株9502-7。对9502-7菌株孢子采用紫外线处理,得到变异高产菌株9502-7-12,其相对效价较出发菌株提高50%以上。     

紫外线与亚硝酸钠复合诱变选育L-组氨酸产生菌

以1株谷氨酸棒杆菌(Corynebacterium glutamicum)S_6作为出发菌株,利用亚硝酸钠(NaNO_2)、紫外线(UV)进行诱变,通过实验证明亚硝酸钠诱变时间在180 s后致死率达到80%,紫外线在照射30 s后致死率达到80%。诱变后的突变菌株经6-巯基嘌呤结构类似物的抗性平板筛选,最终筛得3株菌,Y_1产L-组氨酸量达到331 mg/L,比出发菌株S_6高了5.08%,Z_2产L-组氨酸量达到325 mg/L,比出发菌株S_6高了1.9%,F_6产L-组氨酸量达到330 mg/L,比出发菌株S_6高了7.14%。结果显示,经紫外线与亚硝酸钠复合诱变后的菌株F_6产L-组氨酸的产量最高,比亚硝酸钠诱变后的菌株产L-组氨酸量提高2.06%,比紫外线诱变后的菌株产L-组氨酸量提高5.24%。     

The use of cellulases from a beta-glucosidase-hyperproducing mutant of Trichoderma reesei in simultaneous saccharification and fermentation of wheat straw

Conidia of the cellulolytic strain Trichoderma reesei F522 were mutagenized with UV irradiation and N-methyl|-N'-nitro-N-nitrosoguanidine (NTG). A visual agar plate detection system was developed, using esculin and ferric ions, to identify mutants of T. reesei with increased beta-glucosidase activity. Selected mutants were tested for production of extracellular cellulases in shake flasks on autohydrolyzed wheat straw as carbon source. The most active mutant V-7 showed about 6-times higher activity of beta-glucosidase than the parent strain F-522, whereas the filter paper degrading and endo-1,4-beta-D-glucanase activities increased by 45% and by almost 31%, respectively. Cellulase preparations obtained from the parent and mutant strains were then used along with Kluyveromyces fragilis cells for ethanol production from ethanol-alkali pulped straw in the simultaneous saccharification and fermentation (SSF) process. From 10% (w/v) of straw pulp (dry matter), 2.5% (w/v) ethanol was obtained at 43 degrees C after 48 h using cellulase derived from the parent strain of T. reesei. When the beta-glucosidase-hyperproducing mutant V-7 was employed, the ethanol yield in the SSF process increased to 3.4% (w/v), the reaction time was shortened to 24 h and no cellobiose was detected in straw hydrolyzates.