甘草内生细菌的分离及拮抗菌株鉴定

从乌拉尔甘草健康植株的根茎叶中共分离到内生细菌98株,经初步鉴定芽孢杆菌属（Bacillus sp.）为优势种群,约占30%;从不同生长年份甘草的根、茎、叶组织中分离内生细菌种群密度从5.0×10⁴ cfu/g～2.9×10⁷ cfu/g鲜重不等。采用平板对峙方法筛选出6株对植物病原菌有明显体外拮抗活性的菌株,通过菌落、菌体形态观察、生理生化反应及16S rDNA序列分析,同时结合Biolog细菌自动鉴定系统验证,鉴定这6株拮抗菌分属萎缩芽孢杆菌(Bacillus atrophaeus)、多粘类芽孢杆菌(Paenibacillus polymyxa)、枯草芽孢杆菌(Bacillus subtilis)、Paenibacillus ehimensis。     

抑制铜绿假单胞菌和金黄色葡萄球菌生物膜形成的乳杆菌筛选及机制初探

筛选得到对慢性创面中铜绿假单胞菌（Pseudomonas aeruginosa）和金黄色葡萄球菌(Staphylococcus aureus)生物膜形成具有抑制作用的乳杆菌(Loctobacillus)。测定不同种乳杆菌对铜绿假单胞菌和金黄色葡萄球菌双菌生物膜量、生长及群体感应信号分子AI-2的影响，并采用主成分分析和菌株特性综合分析确定效果最佳的菌株，最后通过荧光定量PCR的方式探究该菌株对生物膜和群体感应相关基因表达的影响。结果表明，植物乳杆菌(Lactobacillus plantarum)、卷曲乳杆菌(Loctobacillus crispatus)、嗜酸乳杆菌(Loctobacillus acidophilus)、鼠李糖乳杆菌(Loctobacillus rhamnosus)、瑞士乳杆菌(Loctobacillus helveticus)、短乳杆菌(Loctobacilkus brevis)具有不同程度的抑菌、抑制生物膜形成的能力，且同种不同株的乳杆菌抑制生物膜形成的能力也有所差异。其中，植物乳杆菌CCFM233产生的AI-2信号分子较多，具有良好的抑菌能力，可使致病菌生物膜形成量降低，铜绿假单胞菌的LasR和rhlI基因表达水平和金黄色葡萄球菌的SarA基因表达水平显著下调。本研究旨在揭示植物乳杆菌CCFM233具有抗铜绿假单胞菌和金黄色葡萄球菌感染的潜力，为其应用于慢性创面敷料提供参考。     

天山大峡谷原始森林黏细菌的分离鉴定及其抗菌活性

【背景】黏细菌是一类具有多细胞群体行为特征的高等原核生物,其对植物病原真菌和细菌的捕食特性使其在植物病害防治方面具有重要的应用潜力。【目的】探究乌鲁木齐天山大峡谷原始森林可培养黏细菌的多样性并分析其抗菌活性,为发掘黏细菌生防菌株奠定基础。【方法】以天山大峡谷原始森林采集的土样和腐木为分离材料,采用兔粪诱导法和被捕食菌诱导法从中分离纯化黏细菌菌株,结合形态学观察、生理生化测定和16S rRNA基因序列分析确定其分类地位,并以6种植物病原真菌[大丽轮枝菌(Verticillium dahliae)、尖孢镰刀菌萎蔫专化型(Fusarium oxysporum f. sp. vasinfectum)、拟轮枝链孢霉(Fusarium verticillioides)、立枯丝核菌(Rhizoctonia solani)、黄色镰刀菌(Fusarium culmorum)、细极链格孢菌(Alternaria tenuissima)]和1种植物病原细菌[梨火疫病菌(Erwinia amylovora)]为靶标菌,通过平板对峙法和菌苔捕食法测定其抗菌活性。【结果】从采集的样品中分离出70株菌株,经纯化后获得36株黏细菌纯培养物。经鉴定隶属于4个属,黏球菌属(Myxococcus) 30株、孢囊杆菌属(Cystobacter) 3株、珊瑚球菌属(Corallococcus) 2株和原囊菌属(Archangium) 1株。抗菌活性分析显示,本研究获得的36株黏细菌至少对2种植物病原真菌有抗菌活性,表现出广谱的抗真菌活性,初步筛选出一株菌株NSE37-1兼具广谱和高效抗真菌活性;供试的15株黏细菌对梨火疫病菌均具有捕食活性,初步筛选出一株对梨火疫病菌具有较强捕食能力的黏细菌菌株NSE25。【结论】天山大峡谷可培养黏细菌资源比较丰富,黏球菌属是该地区可培养黏细菌菌群中的优势菌。分离纯化出的黏细菌菌株均表现出广谱的抗植物病原菌活性,具有进一步研究和开发的潜在价值。     

新疆伊犁野生阿魏菇菌株的分离鉴定与培养特性

对采自新疆伊犁的两种具有不同形态特征的野生阿魏菇（Pleurotus ferulae）子实体分离的菌株进行鉴定和系统发育分析,并探讨优良菌株的培养特性。结合子实体形态和生境特征,利用rDNA-ITS序列,对伊犁野生阿魏菇菌株YL-A1和YL-A2进行分子鉴定及系统发育分析。对阿魏菇菌株YL-A1生长温度、pH、碳源、氮源和无机盐进行单因素试验,分析各因素对菌丝生长的影响,通过L₉(3⁴正交试验,筛选各因子之间的最优组合。结果表明,野生阿魏菇菌株YL-A1（ITS序列GenBank登录号：MN460317）和YL-A2（ITS序列 GenBank登录号：MN809132）,不仅子实体形态特征有差异,且菌株YL-A1菌丝生长速度和长势优于YL-A2,并相互拮抗。结合生境和形态特征及rDNA ITS序列分析,将二者鉴定为阿魏菇(Pleurotus eryngii var. ferulae)。系统发育分析发现,菌株YL-A1和YL-A2单独聚为一组,与其他阿魏菇菌株有一定的遗传距离。经单因素和正交试验,确定了菌株YL-A1在含葡萄糖20 g/L、蛋白胨4 g/L、KH₂PO₄ 1 g/L,pH 7.5的培养基中,25 ℃培养,菌丝生长状态最佳,确定了优良菌株YL-A1菌丝生长最佳培养条件。为进一步保护利用伊犁野生阿魏菇菌种资源提供参考。     

新疆饼干衣属地衣分类学研究

该研究以采自新疆的100余份饼干衣属(Rinodina)地衣标本为研究材料,通过形态解剖特征观察、地衣化学成分分析以及分子生物学鉴定方法鉴定出9个种,包括2个中国新记录种——阿富汗饼干衣(Rinodina afghanica)和古氏饼干衣(Rinodina guzzinii),7个常见种分别是：包氏饼干衣(R. bohlinii)、毕氏饼干衣(R. bischoffii)、代谢饼干衣(R. metaboliza)、密果饼干衣(R. pycnocarpa)、特雷氏饼干衣(R. trevisanii)、甘肃饼干衣(R. straussii)和地生饼干衣(R. terrestris)。并提供了新疆饼干衣属地衣的分种检索表、每个物种的详细描述、新记录种的特征图片以及系统发育分析。     

石鲽病原琼氏不动杆菌形态型Ⅰ的鉴定*

从由杀鲑气单胞菌(Aerom onas salmonicida)所引起的石鲽(Stone flounder,Kareiusbicoloratus L.)细菌性败血感染症病(死)鱼肝、脾、肾及肠内容物中,同时检出了作为继发感染的病原菌。经对6株纯培养菌在形态特征、理化特性等方面较系统的表观分类学指征鉴定及代表菌株DNA中G+C mol%的测定,表明为琼氏不动杆菌的一个新形态型并定名为琼氏不动杆菌形态型Ⅰ(Acinetobacter juniimorphovarⅠ);     

拮抗植物病原真菌的纤维素/木质素降解菌株的筛选及鉴定

【背景】秸秆还田在改善土壤肥力和丰富营养等方面有重要作用,但是也存在秸秆难以快速降解利用和病原真菌病害威胁的问题。【目的】为解决还田秸秆的降解和病原真菌病害问题,从长期秸秆还田地区采集样品,从中筛选出具有降解秸秆和抑菌功能的菌株。【方法】采用稀释分离法、苯胺蓝染色法和刚果红染色法等对秸秆高效降解菌株进行筛选,通过16S rRNA基因测序及构建系统发育树进行菌株鉴定。采用对峙培养法测定筛选到的秸秆降解菌株对玉米大斑病菌(Setostphaeria turcica)、梨黑斑病菌(Alternaria kikuchiana)、马铃薯早疫病菌(Alternaria solani)、链格孢属真菌(Alternaria alternata) ACCC38230和ACCC38231等5种供试植物病原真菌的抑制作用。以玉米大斑病菌(Setostphaeria turcica)为后期供试植物病原真菌,测定拮抗菌株代谢产物的抑菌能力;通过观察拮抗菌株粗提液对玉米大斑病菌分生孢子萌发和菌丝生长的影响,从而测定菌株对病原真菌的抑制作用。【结果】从秸秆还田土壤中分离筛选获得3株高效降解纤维素及木质素菌株并命名为JY122、ZY133和JY215。通过形态学观察和16S rRNA基因测序鉴定上述菌株全部为芽孢杆菌属(Bacillus)。通过系统发育树分析结果表明,JY122与蜡样芽孢杆菌(Bacillus cereus)相似性为99.4%,ZY133与枯草芽孢杆菌(Bacillus subtilis)相似性为100%,JY215与贝莱斯芽孢杆菌(Bacillus velezensis)相似性为99.1%。平板对峙实验结果显示,JY122、ZY133和JY215菌株对不同种属的植物病原真菌均有较强的抑制作用,抑制率高达43.74%-67.54%。此外,上述芽孢杆菌代谢产物具有抑菌活性及很强的热稳定性,经95℃处理后依然具有良好的抑菌效果。【结论】筛选获得的JY122、JY133和JY215菌株具有高效降解纤维素/木质素能力,抑制多种植物病原真菌生长,代谢产物抑菌能力强且热稳定性高。这为玉米秸秆还田提供菌株资源,也为进一步解决秸秆还田难点提供了新方法和思路。     

花生根际微生物的分离及高效功能菌株筛选

【背景】花生根际分布着丰富的微生物类群，分离筛选多种功能的高效微生物是研发高效复合菌肥的基础。【目的】从花生根际土壤及根表分离微生物，分析可培养微生物的多样性，筛选高效解有机磷和无机磷、产吲哚乙酸(indole-3-acetic acid, IAA)和铁载体功能的菌株，为研发花生微生物菌肥打下基础。【方法】利用稀释涂布法，从采自山东省栖霞市、平度市、烟台市莱山区 3个样点的花生根际土、根表样品中分离微生物，基于16S rRNA基因序列对其进行系统发育分析，并通过初筛和复筛筛选高效解磷、产IAA和铁载体的菌株。【结果】共分离、纯化、保藏147株菌，其中75株分离自根际土壤，72株分离自根表样品。系统发育分析表明所有的菌分布于放线菌门(Actinomycetota)、芽孢杆菌门(Bacillota)、拟杆菌门(Bacteroidota)和假单胞菌门(Pseudomonadota)这4个门的40个属，优势属为链霉菌属(Streptomyces, 21.77%)、芽孢杆菌属(Bacillus, 16.33%)；根表样品微生物的多样性高于根际样品；共筛选到解有机磷菌株62株，短波单胞菌(Brevundimonas) YTU21021解有机磷能力最强为1.12 mg/L；解无机磷菌株31株，不动杆菌(Acinetobacter) YTU21009解无机磷能力最强为7.04 mg/L；产IAA的菌株63株，肠杆菌(Enterobacter) YTU21054产IAA量最高，达184.19 mg/L；产铁载体细菌7株，伯克氏菌(Burkholderia) YTU21051产铁载体能力最强，A_s/A_r为0.90。【结论】花生根际和根表样品中可培养微生物多样性较为丰富，本研究筛选到的高效功能菌丰富了花生根际功能微生物资源，为后续与高效根瘤菌联合研发花生复合微生物菌肥奠定了基础。     

基于多位点序列分型对新疆伊宁学龄儿童肠道两歧双歧杆菌(Bifidobacterium bifidum)群体遗传差异解析

【背景】两歧双歧杆菌(Bifidobacterium bifidum)是专性代谢人体母乳寡糖(human milk oligosaccharides, HMOs)和宿主肠道黏膜上皮黏蛋白聚糖的肠道共栖益生菌,对生命早期健康和发育至关重要,目前对其不同人群来源的群体遗传报道较少。【目的】探究在有限地域内遗传、饮食相近人群来源的B. bifidum菌株集的遗传结构是否具有族群特异的规律性,为开发个性化的益生菌株提供理论基础。【方法】对来自新疆伊宁两个族群(维吾尔族和哈萨克族)学龄儿童队列的肠道两歧双歧杆菌进行分离和鉴定,共获得115个菌株,对基于细菌基因组重复序列PCR (repetitive sequence-PCR, rep-PCR)方法筛选的53株代表菌株采用多位点序列分型(multilocus sequence typing, MLST)进行群体遗传差异分析。【结果】53株代表菌株共分为37个序列型(sequence type, ST),具有很高的遗传多样性;其中26株源自维吾尔族儿童的菌株有17个ST,而20个ST来自27株哈萨克族儿童的菌株,两个族群来源的菌株之间检测到较少的同源基因重组事件。goeBURST分析显示,来自同一族群的B. bifidum分离株比来自另一族群的菌株更有可能被归入特定的系统发育分支或克隆复合体(clonal complexes, CC)。【结论】不同族群来源的B. bifidum分离株显示出较高的遗传多样性,群体遗传结构一定程度上呈现出民族族群来源的特异性,需要更大规模的取样证实。这为进一步开展体内外实验并筛选针对区域族群的特色优良益生菌株提供了理论基础。     

牛巴氏杆菌病多重PCR检测技术的建立与应用

【背景】牛巴氏杆菌病是由血清型(A、B、E)多杀性巴氏杆菌(Pasteurella multocida,Pm)引起的一种严重危害养牛业的重要传染病,病原学聚合酶链反应(polymerase chain reaction,PCR)方法是诊断并防控该病的有效手段。【目的】建立检测血清型(A、B、E)多杀性巴氏杆菌的多重PCR方法,为临床诊断牛巴氏杆菌病和病原分型提供技术支撑。【方法】参考多杀性巴氏杆菌hyaD-hyaC基因、bcbD基因和ecbJ基因特异区域,设计3对特异性引物,以温度梯度PCR法确定适宜退火温度(T_m);采用棋盘试验优化引物浓度并初步建立多重PCR方法;采用重组质粒标准品及阳性菌株菌液确定其敏感性(最小检测量);以8种常见牛感染病原体[溶血性曼氏杆菌(Mannheimia hemolytica)C1655、大肠埃希氏菌(Escherichia coli)C237、产单核细胞李氏杆菌(Listeria monocytogenes)C1597、金黄色葡萄球菌(Staphylococcus aureus)C3053、都柏林沙门氏菌(Salmonella dublin)C79351、副结核分枝杆菌(Mycobacterium paratuberculosis)C1625、牛传染性鼻气管炎病毒(bovine infectious rhinotracheitis virus)CAV1546和牛支原体分离株(Mycoplasma bovis)C65-1]核酸样本确定其特异性;制备3批诊断试剂,对敏感性和特异性样品进行批间和批内试验,确定其重复性;运用建立的方法使用3种不同型号的PCR仪检测敏感性和特异性样品,确定其适用性;通过检测临床样本及人工模拟感染样本评价临床应用效果。【结果】在T_m为55℃时,3对引物浓度分别为0.25、0.30和0.20μmol/L条件下建立多重PCR方法较优,可以同时检测多杀性巴氏杆菌血清A型(821bp)、血清B型(203bp)和血清E型(363bp);该方法敏感性高,对重组质粒标准品pMD-A、pMD-B和pMD-E检测限分别为43.080、3.710和4.350copies/μL,对阳性菌液最低检出限均为10²CFU细菌;其特异性强,仅对血清型(A、B、E)多杀性巴氏杆菌有特异性扩增条带,同时对其他病原体均无扩增条带;该方法重复性良好,批间与批内试验均一致;临床样本及人工模拟感染样本检测结果显示与病原分离鉴定符合率为100%。【结论】成功建立了一种可鉴定不同血清型的牛多杀性巴氏杆菌多重PCR检测方法。     

Evolutionary relationships in the genus Bordetella

The nucleotide sequence of the pertussis toxin operon of Bordetella pertussis, Bordetella parapertussis and Bordetella bronchiseptica, has shown that the last two species contain many common mutations and are likely to derive from a common ancestor (Arico and Rappuoli, 1987). To elucidate further the evolutionary relationships between the Bordetella species, we have cloned and sequenced the promoter region and the gene coding for the S1 subunit of pertussis toxin from additional B. pertussis strains, such as the type strain BP 18323 and two recent clinical isolates, namely strain BP 13456 from Sweden and strain BP SA1 from Italy. While the strains BP SA1 and BP 13456 are shown to differ from the published B. pertussis sequences by only one base pair, the type strain BP 18323 contains a total of 11 base-pair substitutions. Remarkably, 9 of the 11 substitutions found in BP 18323 are also common to B. parapertussis and B. bronchiseptica, strongly suggesting that this strain derives from the same ancestor as B. parapertussis and B. bronchiseptica. Computer analysis of the sequence data allows the construction of an evolutionary ‘tree’ showing that the B. pertussis strains are very homogeneous and significantly distant from B. parapertussis and B. bronchiseptica. Therefore the proposed conversion from B. parapertussis to B. pertussis appears highly improbable.     

Representational difference analysis identifies a strain-specific LPS biosynthesis locus in Bordetella spp.

Bordetella pertussis and B. bronchiseptica are genetically very closely related but differ significantly in their virulence properties. Using Representational Difference Analysis (RDA), 11 DNA fragments specific for B. pertussis Tohama I or B. bronchiseptica BB7865 were identified. All B. bronchiseptica BB7865-derived fragments also hybridized with chromosomal DNA from B. parapertussis but not from the B. pertussis strains Tohama I and W28, underlining the close phylogenetic relationship between B. bronchiseptica and B. parapertussis. The B. pertussis type strain BP18323 is a special case, as it contains DNA sequences characteristic for both B. pertussis and B. bronchiseptica. As demonstrated by pulsed-field gel electrophoresis, several of the BB7865-derived fragments are present on a single 30-kb XbaI fragment. Based on the sequences of putative coding regions, four of these fragments may code for proteins involved in carbohydrate metabolism or transport. In agreement with this notion, a mutant for one of these loci synthesizes a significantly altered lipopolysaccharide that lacks the O-specific side chains. The analysis of the corresponding genomic region in various Bordetella species showed that this locus is present in B. bronchiseptica and B. parapertussis but not in B. pertussis. This confirms that the RDA approach has identified a novel strain-specific LPS biosynthesis locus which accounts for the differences between the LPS structures elaborated by different Bordetella species. Received: 24 February 1999 / Accepted: 17 May 1999     

Identification and Cloning of waaF (rfaF) from Bordetella pertussis and Use To Generate Mutants of Bordetella spp. with Deep Rough Lipopolysaccharide

A DNA locus from Bordetella pertussis capable of reconstituting lipopolysaccharide (LPS) O-antigen biosynthesis in Salmonella typhimurium SL3789 (rfaF511) has been isolated, by using selection with the antibiotic novobiocin. DNA within the locus encodes a protein with amino acid sequence similarity to heptosyltransferase II, encoded by waaF (previously rfaF) in other gram-negative bacteria. Mutation of this gene in B. pertussis, Bordetella parapertussis, and Bordetella bronchiseptica by allelic exchange generated bacteria with deep rough LPS phenotypes consistent with the proposed function of the gene as an inner core heptosyltransferase. These are the first LPS mutants generated in B. parapertussis and B. bronchiseptica and the first deep rough mutants of any of the bordetellae.     

Molecular Evolution of the Two-Component System BvgAS Involved in Virulence Regulation in Bordetella

The whooping cough agent Bordetella pertussis is closely related to Bordetella bronchiseptica, which is responsible for chronic respiratory infections in various mammals and is occasionally found in humans, and to Bordetella parapertussis, one lineage of which causes mild whooping cough in humans and the other ovine respiratory infections. All three species produce similar sets of virulence factors that are co-regulated by the two-component system BvgAS. We characterized the molecular diversity of BvgAS in Bordetella by sequencing the two genes from a large number of diverse isolates. The response regulator BvgA is virtually invariant, indicating strong functional constraints. In contrast, the multi-domain sensor kinase BvgS has evolved into two different types. The pertussis type is found in B. pertussis and in a lineage of essentially human-associated B. bronchiseptica, while the bronchiseptica type is associated with the majority of B. bronchiseptica and both ovine and human B. parapertussis. BvgS is monomorphic in B. pertussis, suggesting optimal adaptation or a recent population bottleneck. The degree of diversity of the bronchiseptica type BvgS is markedly different between domains, indicating distinct evolutionary pressures. Thus, absolute conservation of the putative solute-binding cavities of the two periplasmic Venus Fly Trap (VFT) domains suggests that common signals are perceived in all three species, while the external surfaces of these domains vary more extensively. Co-evolution of the surfaces of the two VFT domains in each type and domain swapping experiments indicate that signal transduction in the periplasmic region may be type-specific. The two distinct evolutionary solutions for BvgS confirm that B. pertussis has emerged from a specific B. bronchiseptica lineage. The invariant regions of BvgS point to essential parts for its molecular mechanism, while the variable regions may indicate adaptations to different lifestyles. The repertoire of BvgS sequences will pave the way for functional analyses of this prototypic system.     

Pertactin antigens extracted from Bordetella pertussis and Bordetella bronchiseptica differ in the isoelectric point

Pertactin, which is a membrane-associated antigen of Bordetella pertussis and which is present in many acellular vaccines against whooping cough, has been reported to be similar to the homologous protein in Bordetella bronchiseptica. By running parallel experiments using proteins derived from the two species, we show that the isoelectric point of pertactin from B. pertussis is lower than reported and clearly distinguishable from the homologous protein of B. bronchiseptica. Received: 9 April 1997 / Accepted: 20 May 1997     

Purification, spectroscopic analysis and biological activity of the macrocyclic dihydroxamate siderophore alcaligin produced by Bordetella pertussis and Bordetella bronchiseptica

Hydroxamate siderophores of virulent Bordetella pertussis and Bordetella bronchiseptica strains were purified using a simple large-scale isolation procedure, and identified by various spectroscopic techniques as the macrocyclic dihydroxamate siderophore trivially known as alcaligin, 1,8(S),11,18(S)-tetrahydroxy-1,6,11,16-tetraazacycloeicosane-2,5,12,15-tetrone, which was previously isolated from the taxonomically-related bacterial species Alcaligenes denitrificans subsp. xylosoxydans. Alcaligin purified from iron-depleted cultures of B. pertussis and B. bronchiseptica exhibited specific growth-promoting activity under iron-restricted conditions for Bordetella indicator strains, and were active in [⁵⁵Fe]ferric alcaligin transport assays. Evidence suggests that several C ₂-symmetric conformations of alcaligin exist simultaneously in both methanolic and aqueous solution.     

Expression of urease does not affect the ability of Bordetella bronchiseptica to colonise and persist in the murine respiratory tract

To investigate the role played by urease during the Bordetella bronchiseptica infection process, the ability to colonise and persist in the mouse respiratory tract of a urease-negative B. bronchiseptica BB7865 and a BB7865 derivative constitutively expressing urease was compared with that of the wild-type strain. The results obtained showed that neither constitutive expression nor abolishment of urease activity had any significant effect on the course of B. bronchiseptica infection. Therefore, under our experimental conditions, urease is not essential for B. bronchiseptica to colonise and persist within the murine host.