L-丝氨酸高产菌株的选育和摇瓶发酵条件优化

采用B revibacterium flavmC-11A为出发菌株,经紫外线照射和亚硝基胍诱变处理,选育出一株L-丝氨酸高产菌株C32为目的突变株,使摇瓶产酸率由12.1 g.L-1增加到16.4 g.L-1,然后对其进行摇瓶发酵条件优化,使菌株C32的L-丝氨酸产率提高到30.1 g.L-1。     

L-苯丙氨酸产生菌的选育

本文报导了不产酸的谷氨酸棒杆菌(Corynebacteriumglutamicum)经亚硝基胍处理,在一定浓度的L-苯丙氨酸结构类似物——对氟苯丙氨酸(DLP-Fluorophenylalalline,PFP)存在下,筛选获得了一批能产生与积累L-苯丙氨酸的抗代谢突变菌株,其中PFP-17突变菌株的产物在纸层析谱上L-苯丙氨酸的显色点较深,定量测定产酸为1.5mg/ml经两次自然分离获得的17-3-4菌株产酸特性稳定,在以葡萄糖为主要碳源,初糖为4.5%的摇瓶发酵中。产酸可达5.5mg/ml,产物经氨基酸自动分析代鉴测确证其主要产物是L-苯丙氨酸,此突变菌株经进一步选育所得的突变菌株3-PAP-42在提高初糖为6%时,发酵产酸可达8.28mg/ml。     

L-缬氨酸高产菌株的选育研究

以产L-缬氨酸的谷氨酸棒状杆菌(Corynebacterium glutamicum)为原始菌株,利用注入低能氮离子束进行一系列诱变,获得一株稳定的高产L-缬氨酸突变菌株。摇瓶培养96h后发酵能力可达38.0g·L-1,较出发菌株提高18.01%。通过对摇瓶中葡萄糖、玉米浆浓度及培养条件进行优化,发酵能力达到40.6g·L-1,50L发酵罐的发酵能力可达70g·L-1左右。     

耐温性L-谷氨酸发酵菌种的选育

应用基因组改组技术提高,L-谷氨酸生产菌在高温发酵条件下的谷氨酸产量。以天津短杆菌T6—13变异株SW07-1为原始亲株,分别经紫外线（UV）-硫酸二乙酯（DES）和X射线诱变,获得5株耐温性能略有提高的突变菌株。经2轮基因组改组,获得耐高温（能在44℃生长）的L-谷氨酸菌株F2-50。F2—50在38℃下,摇瓶发酵40h,发酵液中L-谷氨酸浓度比原始出发菌株提高了近41％,在41℃高温下,摇瓶发酵40h,L-谷氨酸浓度比原始出发菌株提高了近2倍。     

L-异亮氨酸产生菌的选育

以黄色短杆菌BF420为出发菌株,经紫外线和亚硝基胍复合诱变处理后,单菌落分离筛选到一株营养缺陷型突变菌株BF35(Lys-).进一步采用氨基酸结构类似物S-2-氨基乙基-L-半胱氨酸(AEC)、α-氨基丁酸(α-AB)进行抗性筛选,获得一株带有遗传标记的L-异亮氨酸高产突变株BF3510(Lys-+AECr +a-ABr).该菌株在培养基未优化的条件下摇瓶产酸量为6.4g·L-1,比出发菌株增加了83％.     

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。     

PGDH~L生化突变型谷氨酸生产菌株选育的生化模式

以Tbm-3（icl-,异柠檬酸裂解酶活力丧失的生化突变株）为出发菌株,经紫外线诱变,通过依据生化代谢所设计的选择培养基（L-阿拉伯糖平板与D-葡萄糖酸钠平板）对接的筛选方法,获得磷酸葡萄糖酸脱氢酶（PGDH,E．C．4．2．1．12）渗漏突变型（pgdh1）的生化突变型菌株Tbm3-18．该菌株经摇瓶发酵试验显示,比出发菌株Tbm-3提高产酸率8．9％和转化率8．1％．表明pgdh-或pgdh1生化突变型菌株的选育,对谷氨酸的积累是有利的,该选育生化模式是成功的．     

L-精氨酸产生菌诱变育种的研究

本文报道了L-精氢酸产生菌诱变育种的研究结果。以谷氨酸产生菌钝齿棒状杆菌AS1．542为出发菌株,经亚硝基胍多次逐级诱变,获得了一株能够积累大量L-精氨酸的菌株971.1。该菌属于组氢酸缺陷型,并具有对磺胺孤的抗药性。在以葡萄糖为碳源、硫酸铵为氮源的培养基中直接发酵四天,产酸最高可达25·2 mg／ml,并具有较高的产酸稳定性。     

抗噬菌体谷氨酸高产菌株选育

从污染的谷氨酸发酵废液中分离纯化噬菌体,并以高滴定度侵染生产敏感菌,借助菌的自发突变筛选出抗噬突变株,再运用紫外线、亚硝基胍复合诱变手段经过初筛、复筛,最后选育出抗噬谷氨酸高产菌株。其过程简单、便利,可靠性高,是选育抗噬谷氨酸高产菌株的好方法,对发酵行业具有指导意义。曾选育到抗噬谷氨酸高产菌株,其摇瓶发酵产量比对照提高26.4%。     

L-苹果酸产生菌筛选及高产突变株诱变选育

通过广泛收集和分离,获得根霉属(Rhizopus)、曲霉属(Aspergillus)及裂褶菌属(Schizophyllum)等属菌株897株。产酸指示平板上的变色圈测定结果表明,它们中间628株为产酸菌。通过纸层析对产酸菌发酵液酸谱的分析,获得129株L-苹果酸产生菌,经进一步测定发酵液中L-苹果酸的含量,筛选出以葡萄糖为原料,摇瓶发酵140小时,L-苹果酸产率48．37g／L,对糖转化率48．37×10^-2 的菌株LMO2。经初步鉴定,这一菌株为曲霉(Asper-gillus sp.)以LM02作为出发株,采用亚硝基胍、自然污染细菌、甲基磺酸乙酯及紫外线进行诱变处理,选育出葡萄糖为原料,L-苹果酸产率较高的突变抹N1-14、N1-14、NE1412、NU1416及NU1419。其中N1-14 的L-苹果酸产量最高,比出发株提高46．2×10^-2。N1-14 的菌丝生长速度快,产孢能力强,摇瓶发酵葡萄糖140小时,平均L-苹果酸产率为72．53g／L,对糖转化率53．74×10^-2。全发酵液经薄层层析测定,不含黄曲霉毒素。发酵产物分离提纯后,得到白色粉末状结晶,经纸层析、质谱及红外光谱测定,证明为L-苹果酸。     

phbC基因敲除对土壤杆菌产可得然胶的影响

本文构建了phbC基因无痕敲除菌株ΔphbC,分析了ΔphbC菌株生长代谢情况和产生的可得然胶在产量、凝胶性质和红外结构的变化。结果显示,ΔphbC菌株在发酵过程中氨基氮消耗情况与野生型菌株一致,在蔗糖消耗方面,ΔphbC菌株与野生型菌株在18 h之后出现显著差异,蔗糖消耗比野生型菌株明显降低。ΔphbC菌株可得然胶产量约24 g/L,相对于野生型菌株降低了45%;胶凝胶强度为812.521 g/cm^2,相对于野生型菌株降低了21%;红外结构与野生型菌株一致,无明显差异。phbC基因不影响菌体生长,不影响可得然胶结构,但是影响可得然胶的合成。     

灰黄霉素菌的诱变效应

以灰黄霉素产生菌D－756为出发菌株,经过三代紫外线＋氯化锂诱变处理,获得耐氯变株F－1012,该变株在形态特征及产量、耐氯性等方面均发生变化,当发酵培养基中的氯化物浓度由1.5%提高到2.0%,F－1012的大米孢子效价提高了34.5%;当固体平板培养基中氯化物浓度提高到11％时,F－1012的孢子存活率比出发菌株提高了25.5％。     

Transductional construction of a threonine-producing strain of Serratia marcescens.

A threonine-producing strain of Serratia marcescens Sr41 was constructed according to the following process. Thr- strain E-60 was derived from strain HNr59 having constitutive levels of threonine-sensitive aspartokinase and homoserine dehydrogenase. Thr+ transductant T-570 was constructed from strain E-60 and phage grown on strain HNr21 having feedback-resistant threonine-sensitive aspartokinase and homoserine dehydrogenase. This transductant lacked both feedback inhibition and repression for the two enzymes. Thr- strain N-11 was derived from strain AECr174 lacking feedback inhibition and repression of lysine-sensitive aspartokinase. Subsequently, the threonine region of strain T-570 was transduced into strain N-11. One of the THR+ transductants, strain T-693, produced markedly high levels of the two aspartokinases and homoserine dehydrogenase, which were insensitive to feedback inhibition. This strain produced about 25 mg of threonine per ml in the medium containing sucrose and urea.     

Transductional construction of a threonine-producing strain of Serratia marcescens.

A threonine-producing strain of Serratia marcescens Sr41 was constructed according to the following process. Thr- strain E-60 was derived from strain HNr59 having constitutive levels of threonine-sensitive aspartokinase and homoserine dehydrogenase. Thr+ transductant T-570 was constructed from strain E-60 and phage grown on strain HNr21 having feedback-resistant threonine-sensitive aspartokinase and homoserine dehydrogenase. This transductant lacked both feedback inhibition and repression for the two enzymes. Thr- strain N-11 was derived from strain AECr174 lacking feedback inhibition and repression of lysine-sensitive aspartokinase. Subsequently, the threonine region of strain T-570 was transduced into strain N-11. One of the THR+ transductants, strain T-693, produced markedly high levels of the two aspartokinases and homoserine dehydrogenase, which were insensitive to feedback inhibition. This strain produced about 25 mg of threonine per ml in the medium containing sucrose and urea.     

Alternation of the Dissimilation Pathway for Glycerol and Amplification of Glycerol Dehydrogenase in Mutant Strains of Cellulomonas sp. NT3060

Mutant strain ME544, which is able to grow on glycerol slowly, was derived from glycerol-negative mutant strain G011, which is a derivative strain of Cellulomonas sp. NT3060 and is defective in both the enzyme activities of glycerol kinase and glycerol 3-phosphate dehydrogenase. The mutant strain still lacked both the enzyme activities involved in the dissimilation of glycerol and had the same level of glycerol dehydrogenase activity as the parent strain. Dihydroxyacetone kinase activity in mutant strain ME544 was inducibly formed, reaching 4-fold the level in mutant strain G011 in glycerol medium. Thus, the mutant strain seemed to dissimilate glycerol by means of glycerol dehydrogenase followed by an increase in dihydroxyacetone kinase. Subsequently, a mutant strain, GP1807, which was resistant to the inhibition of growth on glycerol by 1,2-propanediol, was derived from mutant strain ME544. Glycerol dehydrogenase activity of the mutant strain was amplified about 6-fold compared to that of the wild type strain.     

Cloning and Characterization of the Genomic RNA Sequence of the Mumps Virus Strain Associated with a High Incidence of Aseptic Meningitis

cDNA clones of the mumps virus wild-type strain, associated with a high incidence of aseptic meningitis (ODATE-1 strain), were isolated and analyzed from genomic nucleotide position 22 to 8520 containing the NP, P, M., F, SH and HN protein coding region. The ODATE-1 strain exhibited a RFLP profile identical to that of the Urabe vaccine strain in spite of the fact that the virus was isolated from non-vaccinated cases. However, a comparison of nucleotide and amino acid sequences among the ODATE-1 strain, Urabe strain and Miyahara strain revealed that the ODATE-1 strain was not related to the Urabe strain.     

家蚕近交系遗传纯度的RAPD检测

目的分析家蚕近交系IS-c108A的遗传纯度,为家蚕实验动物化的培育工作提供指导。方法应用经过筛选的20条随机引物对家蚕近交系IS-c108A(F10)的3个蛾区各30个个体和该近交系的亲本系统c108、对照实用化品种871各30个个体的基因组DNA进行RAPD扩增,计算个体间和蛾区间的相似系数及遗传距离。结果家蚕近交系IS-c108A(F10)的3个蛾区内的多态性带频率分别为1.807%、1.841%、1.841%,平均为1.830%;起点亲本c108个体间多态性带频率为7.207%,对照品种871个体间的多态性带频率为7.08%;而近交系IS-c108A与c108之间的多态性带频率为49.20%,c108和871品种之间的多态性带频率为58.33%。家蚕近交系IS-c108A10的3个蛾区内个体之间遗传相似系数的平均值分别为0.99581、0.99555、0.99551,总平均为0.99562。结论家蚕近交系IS-c108A(F10)已具有较高的遗传纯合度,家蚕具有易于获得高纯的有利条件。     

Comparisons of Characteristics of Mercury-Tolerant Bacterium Pseudomonas oleovorans G-1 and Its Mercury-Sensitive Mutant Strain

An Hg²⁺-sensitive mutant strain was isolated from an Hg²⁺-tolerant bacterium Pseudomonas oleovorans G-1 strain by mutagenesis with N-methyl-N′-nitro-N-nitrosoguanidine. The Hg²⁺-sensitive mutant strain was about 10-times as sensitive to Hg²⁺ as the parent strain. Moreover, the mutant strain was considerably more sensitive to Cr⁶⁺ than the parent strain, but it did not show an appreciable change in sensitivity to Cd²⁺ and Cu²⁺. The mutant strain was considerably more sensitive to antibiotics achromycin, chloramphenicol and streptomycin than the parent strain. A more rigid structure was observed in the cell envelope of the mutant strain than the parent strain under transmission electron microscope. Higher amounts of DNA but less protein and RNA were found in the mutant strain compared to the parent strain. Disc electrophoretic patterns showed some differences in protein bands between the parent and mutant strain.     

在乳酸乳球菌中表达外源谷氨酰胺转胺酶显著改善宿主菌好氧生长性能

为改善乳酸乳球菌的生长性能,以轮枝链霉菌染色体DNA为模板,扩增得到编码谷氨酰胺转胺酶成熟酶的基因mtg,将其克隆到质粒pNZ8148中,电转化乳酸乳球菌NZ9000,获得乳酸乳球菌NZ9000(pFL001)(重组菌)。在不控制pH条件下,重组菌的胞外pH显著高于对照菌NZ9000(pNZ8148);前者的最高生物量可达4.13gL,而后者只有0.34gL。在控制pH为6.5±0.1的条件下,重组菌最高生物量为4.73gL,对葡萄糖的菌体最高平均得率为71.1gmol,而相同条件下对照菌最高生物量为2.6gL,对葡萄糖的菌体最高平均得率为27.3gmol。由此表明,重组菌与对照菌相比,好氧生长性能得到显著改善。可能的原因是mtg的活性表达升高了重组菌的胞内pH,原先用于泵出胞内H 所需的部分能量可能因此得到节省,这样相应增加了用于细胞生长的能量。