对紫云英根瘤菌突变株的生长情况及产生细胞分裂素能力的考察

紫云英根瘤菌突变株96号,只有增强了原来培养基的缓冲能力并增加了氮源后,才能使其正常生长。96号突变株产生细胞分裂素的能力随着生长过程的不同而异。它产生细胞分裂素的最大量在菌体生长的稳定初期,为15.01μg/L,比出发菌株的2.18 μg/L提高了近7倍。经修改后的根瘤菌常规培养基能用于该菌株的发酵培养,并能正常产生细胞分裂素类物质。在培养液中加入腺嘌呤对菌体合成细胞分裂素类物质有强烈的诱导效应。     

酵母细胞转运正烷烃的研究——Ⅱ.糖类对突变菌株U_(3-21)的生长、乳化剂和二羧酸产生的影响

以不同碳链的正烷烃作为唯一生长碳源时,U_(3-21)菌株产生乳化剂的量不同,因而菌体生长也不同,产生乳化剂多的,菌体生长也好。本文主要报道在烷烃发酵中,糖类对菌株产生乳化剂的促进与抑制怍用,0.15%的蔗糖,大大促进了乳化剂的产生,加速菌体生长,提高二羧酸的产量。发酵培养基初始pH不同,也影响菌体生长和二羧酸产量。     

精氨酸脱亚胺酶发酵过程特性研究

精氨酸脱亚胺酶有较好的体内体外肿瘤生长抑制作用。通过对粪肠球菌（Enterococcus faecalis）NJ402菌株产精氨酸脱亚胺酶的发酵特性的研究,建立起代谢物的过程变化与精氨酸脱亚胺酶产生机理的内在联系。NJ402菌株生长过程中碳源物质代谢产生乳酸导致发酵体系pH的下降,而培养基中L-精氨酸的脱亚胺作用有利于发酵体系pH的稳定和菌体生长。进一步的研究表明,低pH生长环境有利于NJ402菌株产精氨酸脱亚胺酶,且精氨酸脱亚胺酶的产生与能量代谢无关。NJ402菌株产精氨酸脱亚胺酶受底物L-精氨酸的诱导,但该诱导作用受菌体生长体系pH的调控,即精氨酸脱亚胺酶的产生是低pH生长环境与L－精氨酸共同作用的结果。     

铁对产铁载体的沼泽红假单胞菌光合色素与铁载体合成的影响

【目的】探求铁对1株能产生铁载体的不产氧光合细菌(Anoxygenic Phototrophic Bacteria,APB)光合色素和铁载体合成的影响。【方法】通用CAS法检测铁载体产生,Arnow、Csaky和Shenker法检测铁载体类型;吸收光谱法和HPLC法分析光合色素的组分和含量。【结果】Rhodopseudomonas palustris CQV97能够产生异羟肟酸型铁载体,未添加FeCl3时,铁载体含量最高,铁载体的产生与生长并非关联型。随FeCl3浓度升高,菌体生长潜伏期缩短,生长速率、最终生物量以及细菌叶绿素(Bacteriochlorophyll,BChl)a和类胡萝卜素(Carotenoid,Car)含量均提高,而检测到的游离铁载体含量降低;菌体积累的BChl a的组成和相对含量未见明显变化,但主要的Car组分由Spirilloxanthin转化为Rhodopin,菌体中积累Car组分的平均共轭体系降低,Car组成的改变与色素提取液的Car特征性光谱蓝移现象相吻合。【结论】首次报道APB能够产生铁载体,CQV97菌株能够产生异羟肟酸型铁载体。阐明了铁对CQV97生长、铁载体产生和光合色素合成的影响规律,这些研究结果为深入开展APB铁载体分离纯化以及生物功能研究奠定了基础。     

类植物乳杆菌的耐酸、耐胆盐及降胆固醇特性

摘要：【目的】研究了类植物乳杆菌Ⅱ32的酸、胆盐耐受性和胆固醇去除能力,并通过菌株生长和胆固醇去除的关系探讨可能的机理。【方法】菌株Ⅱ32生长在高胆固醇MRS培养基中,胆固醇的检测通过气相色谱法。检测菌株在不同生长阶段对胆固醇的去除情况。【结果】菌株Ⅱ32具有酸耐受性、胆盐耐受性和一定的胆固醇清除能力。菌株在pH2.0培养2 h后仍能达到104 cfu/mL;加胆盐（0.3%～0.4%）对菌株生长量达到OD值0.6的时间延迟在0.5 h以内;热杀死的和休眠的细胞能去除很少的胆固醇,分别是5.64、5.90 mg/g细胞干重,而生长的细胞去除的胆固醇达到16.98 mg/g细胞干重。另外,研究表明胆固醇去除与菌体的生长有一定的相关性。【结论】菌株Ⅱ32去除胆固醇可能的机理是菌体对胆固醇的吸附及菌体在生长过程中对胆固醇的吸收利用,为此该菌株具有添加到食品中来降低血液胆固醇的潜能。     

ppc基因敲除对大肠杆菌L-色氨酸发酵的影响

目的：减少大肠杆菌L-色氧酸前体物质磷酸烯醇式丙酮酸向草酰乙酸的代谢流,提高其L-色氨酸的产量。方法：以大肠杆菌TRTH0709为出发菌株,利用Red重组敲除技术敲除磷酸烯醇式丙酮酸羧化酶（Ppc）编码基因PPc,并经测序和酶活性检测确证;对出发菌株和基因敲除菌株进行L-色氖酸发酵,对比分析发酵结果。结果：测序和酶活性检测结果表明ppc基因被成功敲除。发酵结果表明,与出发菌株相比,基因敲除菌株TRTH0709△ppc生长速度减慢,最终生物量减少32％,L-色氯酸产量降低27％,但糖酸转化率提高6％;向发酵培养基中添加1％琥珀酸后,TRTH0709△ppc的生长速率和产酸量有所提高,但仍与出发菌株有一定差距。结论：虽然ppc基因敲除对菌体生长和产酸量影响较大,但能有效提高其糖酸转化率;选育Ppc弱化的突变株以达到减弱代谢流且不影响菌体生长,以及增加,L-色氨酸积累的目的,将是本研究今后的主要方向。     

培养条件对里氏木霉306菌体形态和t-PA生物合成的影响

里氏木霉（Trichoderrna reesei）306是能够生物合成组织型纤溶酶原激活剂（t-PA）的基因工程菌株。在对其液态深层培养时,发现随培养夸件和培养时间的变化,其菌体能以松散和菌丝球的两种形态存在。菌体形态和t-PA的产生密切相关。培养基中无机盐和表面活性剂的种类和添加量以及接种量和pH等培养条件是影响里氏木霉306菌体形态和t-PA合成的主要因素。在液态深层培养过程中,菌体以松散的菌丝体形态生长,形成纸浆状发酵液,利于t-PA的合成。     

大肠杆菌乙酸代谢突变株的选育和特性研究

在大肠杆菌高密度培养中 ,因代谢副产物乙酸积累 ,导致抑制菌体的生长和产物表达的下降。为减小乙酸的抑制作用 ,采用60 Co诱变处理大肠杆菌JM1 0 1 ,结合连续培养 (含乙酸钠选择压力 )定向富集方法 ,选育到一株乙酸耐受性增强的菌株JL3。该菌株表现出明显的乙酸耐受性的提高 ,在含有 1 0 g/L乙酸钠的MA培养基中 ,菌体生长和葡萄糖消耗速率都有较大程度提高 ,并且具有良好的遗传稳定性     

产生辅酶Q10的光合细菌菌株的分离及鉴定

对水塘污泥中富集分离的13株光合细菌产生的CoQ10进行定性定量分析,筛出CoQ10含量较高的菌株2c并对其进行系统鉴定。菌株2c为革兰氏阴性菌,细胞杆状,菌体大小0.6μm～0.9μm×1.2μm～2.0μm,单极生鞭毛,片层状光合内膜,位于细胞质膜下并与之平行。光照厌氧或黑暗好氧条件下均可生长,光照下菌体产生红色素,菌体含有细菌叶绿素a和类胡萝卜素。最适生长温度30～35℃,pH7.0～8.0。多种有机化合物均可作为光合作用的电子供体和碳源,蛋白胨和硫酸铵是其生长的较好氮源,酵母膏对其生长有明显刺激作用。16S rDNA序列系统发育分析表明,菌株2c在系统进化树上与GenBank中序列号为AY751758、DQ001155、DQ001158的沼泽红假单胞菌聚为一族。菌株2c至少能稳定传代15次。初步确定菌株2c为沼泽红假单胞菌。     

降解菊粉担子菌的分离鉴定及其酶的产生

从菊芋地的腐木上分离到一株在以菊粉为唯一碳源和能源的培养基上生长良好,具有较高菊粉酶活性的担子菌菌株,经鉴定为采绒革盖菌（Ｃｏｒｉｏｌｕｓｖｅｒｓｉｏｌｏｒ）。该菌的菊粉酶大部分是胞外酶,此酶对菊粉的专一性高,其Ｉ／Ｓ比值在发酵过程中不断变化。菊粉酶活性平行地随菌体生长而增加。该酶的合成受菊粉诱导,受果糖抑制。当果糖浓度大于２．７ｍｇ／ｍｌ时,菊粉酶活性为零。菌体的匀质化可使生长加快从而获得大量菊粉酶。     

Role of water activity in ethanol fermentations

A separate role for water activity in the conversion of sugars to ethanol by two strains of yeast is identified. During fermentation of both single and mixed sugar substrates, the water activity was shown to remain constant during the logarithmic growth phase. This is despite the changes in concentration of substrates and product, the constancy reflecting the fact that the greater influence of ethanol on the solution activity is counterbalanced, in the early stages of the fermentation, by its low yield. The end of the log phase of growth coincides with the start of a period of gradually decreasing water activity. For the more ethanol-tolerant strain UQM66Y, growth was found to cease at a constant value of water activity while that for the less tolerant strain UQM70Y depended on both ethanol concentration and water activity. It is argued that water activity is a more appropriate variable than ethanol concentration for describing some of the nonspecific inhibitory effects apparent in ethanol fermentations. A straightforward method for the calculation of water activity during such fermentations based on the use of solution osmolality is presented.     

产细菌素的细菌筛选鉴定及其产物抑菌性能研究

从水体改善制剂样品中筛选出一株产细菌素的芽孢杆菌XDF-2,经生理生化分析和分子生物学鉴定,确定为短小芽孢杆菌。发现该菌产细菌素受发酵时间和培养的影响。对该粗提的细菌素进行特性研究,发现该细菌素只对金黄色葡萄球菌和藤黄微球菌具有抑菌活性。但是该细菌素在不同pH、100℃以下的温度、表面活性剂和有机溶剂的环境下稳定。经酶解试验所得,推测该细菌素具有多肽结构和羧基酯的结构。     

野生灵芝BSU01的分离鉴定、生物学特性及其木质纤维素酶活分析

灵芝作为传统中药,具有重要的医药和经济价值。本研究以一株野生灵芝属真菌BSU01为实验材料,通过形态特征和ITS序列聚类分析对其进行了鉴定,探讨了该菌株菌丝生长的最适碳源、氮源、C/N、pH及温度等生物学特征,以及该菌株产木质纤维降解素酶的能力。结果表明,菌株BSU01的形态特征与有柄灵芝相符;且与有柄灵芝ITS序列一致性达99%,并在系统发育树上聚在一起;菌株BSU01菌丝生长最适碳源为果糖或者葡萄糖,氮源为酵母提取物,C/N比为20/1到30/1,温度为30℃,pH值为5.5;菌株BSU01的漆酶、木质素过氧化物酶和Mn依赖过氧化物酶分别为12.13 U/L、0.52 U/L和0.33 U/L;CMCase和木聚糖酶酶活分别为7.14 U/mL和1.88 U/m L。本研究结果将为该菌的进一步开发利用提供数据参考。     

一株产乙酰酯酶细菌筛选、鉴定及酶学性质研究

【目的】利用筛选培养基,从肉牛瘤胃液中分离筛选产乙酰酯酶的细菌菌株,并研究菌株的产酶特征。【方法】利用厌氧培养技术,以木质素为唯一碳源,筛选并驯化所得菌株。根据菌株16S rDNA序列分析、革兰氏染色、伊红美蓝培养基培养、甲基红试验和柠檬酸盐利用试验,鉴定菌株。采用对-硝基苯乙酯测定酶活力。【结果】筛选得到产乙酰酯酶活力较高细菌菌株RB1,初步鉴定为Escherichia coli。菌株RB1的生长曲线表明,0 42 h为菌株的延迟期,42 60 h为菌株的对数期,60 66 h为菌株的稳定期,66 86 h为菌株的衰亡期。菌株所产乙酰酯酶最适温度为40°C,最适pH为8.0,在最适温度与pH条件下,培养基中添加玉米秸秆粉,乙酰酯酶最高酶活力达到0.52 U/mL。【结论】筛选获得产乙酰酯酶的细菌菌株RB1,其乙酰酯酶活力高于已报道的菌株,是一株具有研究和应用潜力的产乙酰酯酶的菌株。     

Identification of a Fourth Staphylococcal Enterotoxin, Enterotoxin D

A fourth staphylococcal enterotoxin was identified serologically with antiserum to the very crude enterotoxic products of growth of a strain which also produces enterotoxin C, and then with antiserum to the considerably purified enterotoxic antigen of a strain which produces only the new enterotoxin. The identification of this antigen as enterotoxin D was based on the following observations. It was produced by strains which do not produce enterotoxins A, B, or C; it was absent in the growth products of nonenterotoxigenic strains; when appreciably purified, it was associated with emetic activity in the cat, and its biological activity was neutralized only by antisera containing its specific antibody and not by antibodies to enterotoxins A, B, and C. Staphylococcal strain 494 (ATCC 23235) was selected as the prototype strain. The production of this enterotoxin alone and together with enterotoxin A by strains of food-poisoning origin indicates that its role in food poisoning is second in frequency only to that of enterotoxin A. The incidence of production of enterotoxins A, B, C, and D, and of unidentified cat emetic substances by strains from several source categories, is presented.     

汉坦病毒结构蛋白的鉴定及其应用

对差速离心纯化的汉坦病毒R84-1毒株进行了SDS-PAGE和免疫印迹试验。发现有67k和43k两条蛋白区带能与汉坦病毒抗体起反应。经单克隆抗体鉴定,67k多肽可能属病毒囊膜蛋白,43k多肽未定。用免疫印迹法对出血热患者进行检测,初步证明野鼠型感染者具有上述两种蛋白抗原的抗体,大鼠型患者仅具有67k蛋白的抗体,这对出血热患者血清学分型有重要意义。     

低温条件下诱变菌株的营养动力学研究及分子鉴定

以实验室保存的经过低温混合诱导的乳酸菌菌株Q1-4-6为研究对象,通过生长及产酸情况,研究其在低温条件下对于各种营养素的需求,以期为工业大规模生产提供数据参考。低温条件下通过研究碳源对菌株生长及产酸的影响发现,麦芽糖和乳糖对于菌株的生长及产酸有非常好的促进作用,菌株在以蔗糖为碳源的培养基中生长缓慢,而在以乳糖为碳源的培养基中生长最好。3种氮源对于菌株生长的差异不显著,以酵母膏为氮源的菌株生长略好于其他2种。不同浓度金属离子对于菌株生长有不同影响,Zn2+的促生长作用略高于Fe2+,Zn2+浓度越低,菌株生长越好,高浓度的Zn2+则对菌株生长有抑制作用。Fe2+浓度为0.5 g/L时,菌株生长最好,Fe2+浓度过高或过低对于菌株的生长都有抑制作用。根据16S rDNA序列分析结果,同时结合形态学特征、生理生化特性,将菌株鉴定为棉籽糖肠球菌(Enterococcus raffinosus)。     

GTP Hydrolysis Is Not Important for Ypt1 GTPase Function in Vesicular Transport

GTPases of the Ypt/Rab family play a key role in the regulation of vesicular transport. Their ability to cycle between the GTP- and the GDP-bound forms is thought to be crucial for their function. Conversion from the GTP- to the GDP-bound form is achieved by a weak endogenous GTPase activity, which can be stimulated by a GTPase-activating protein (GAP). Current models suggest that GTP hydrolysis and GAP activity are essential for vesicle fusion with the acceptor compartment or for timing membrane fusion. To test this idea, we inactivated the GTPase activity of Ypt1p by using the Q67L mutation, which targets a conserved residue that helps catalyze GTP hydrolysis in Ras. We demonstrate that the mutant Ypt1-Q67L protein is severely impaired in its ability to hydrolyze GTP both in the absence and in the presence of GAP and consequently is restricted mostly to the GTP-bound form. Surprisingly, a strain with ypt1-Q67L as the only YPT1 gene in the cell has no observable growth phenotypes at temperatures ranging from 14 to 37°C. In addition, these mutant cells exhibit normal rates of secretion and normal membrane morphology as determined by electron microscopy. Furthermore, the ypt1-Q67L allele does not exhibit dominant phenotypes in cell growth and secretion when overexpressed. Together, these results lead us to suggest that, contrary to current models for Ypt/Rab function, GTP hydrolysis is not essential either for Ypt1p-mediated vesicular transport or as a timer to turn off Ypt1p-mediated membrane fusion but only for recycling of Ypt1p between compartments. Finally, the ypt1-Q67L allele, like the wild type, is inhibited by dominant nucleotide-free YPT1 mutations. Such mutations are thought to exert their dominant phenotype by sequestration of the guanine nucleotide exchange factor (GNEF). These results suggest that the function of Ypt1p in vesicular transport requires not only the GTP-bound form of the protein but also the interaction of Ypt1p with its GNEF.     

Immunological demonstration of a unique 3,4-dihydroxyphenylacetate 2,3-dioxygenase in soil Arthrobacter strains.

Many bacteria biosynthesize 3,4-dihydroxyphenylacetate 2,3-dioxygenases for growth on aromatic acids, but gram-negative organisms have been most extensively studied. A gram-positive strain containing 2,3-dioxygenase activity was identified as Arthrobacter strain Mn-1. The 2,3-dioxygenase from strain Mn-1 was purified to homogeneity by fast protein liquid chromatography with a Mono Q anion-exchange column. Rabbit polyclonal antidioxygenase antibodies were prepared. Ouchterlony double-diffusion and Western blotting (immunoblotting) protocols were used to probe the distribution of the Mn-1 dioxygenase antigen in soil bacteria. Fourteen 2,3-dioxygenase-containing Bacillus and Pseudomonas strains did not contain immunologically cross-reactive proteins. Six of eight Arthrobacter strains contained 2,3-dioxygenase activity, and all of them produced cross-reactive proteins. The data presented here suggest that a unique type of dioxygenase is geographically widespread but is taxonomically confined to Arthrobacter soil bacteria.