5株海洋微藻伴生细菌的分离鉴定与功能分析

[目的]研究水产养殖中常用的4种海洋微藻在粗放培养过程中所伴生的主要细菌。[方法]采用平板涂布的方法成功分离到5株可培养的海洋细菌,利用16S rRNA基因序列的通用引物对单克隆菌落进行PCR扩增,所得PCR产物经测序和Genbank比对后,采用邻位相接法构建了系统进化树,并对其种属关系进行了分析。[结果]研究表明,5株海洋细菌分属于α-proteobacteria和γ-proteobacteria两大类别。根据16S rRNA基因序列的种属关系分析,5株海洋细菌分属于Porphyrobacter、Devosia、Ponticoccus、Marinobacter和Roseobacter5个属。根据其相近种的生理生化特征推断,这些伴生细菌在分解微藻胞外产物为微藻提供无机营养盐和分泌促生长因子促进微藻的生长等方面可能发挥着重要作用。[结论]在实际的微藻饵料培养过程中,应注意保留这些有益的伴生细菌。     

梭鱼和鲻鱼线粒体16S rRNA和COⅠ基因片段的比较分析

运用PCR技术,扩增了梭鱼和鲻鱼线粒体16S rRNA和COⅠ基因片段,并比较分析了其种间的序列差异。获得16S rRNA基因的540～560 bp碱基序列,出现26个碱基的插入与缺失位点;获得COⅠ基因的602～604 bp碱基序列,出现2个插入缺失位点;16S rRNA和COⅠ基因的序列中G平均含量最低,且（A＋T）含量高于（G＋C）含量,与其他鱼类中的16S rRNA和COⅠ基因片段研究结果相一致。在16S rRNA基因片段中,梭鱼出现1种单倍型,鲻鱼为2种单倍型;在COⅠ基因片段中,梭鱼样品中检测到3个单倍型,鲻鱼样品中检测到5个单倍型。以Takifugu poecilonotus为外群,构建的NJ系统发育树,基于16S rRNA和COⅠ基因序列获得的NJ系统树基本一致,鲻鱼和梭鱼种内个体分别聚为一支,显示16S rRNA和COⅠ基因适合于梭鱼和鲻鱼的物种鉴定。     

副猪嗜血杆菌实时荧光PCR快速检测方法的建立和应用

[目的]建立一种快速准确定量检测副猪嗜血杆菌（HPS）的检测方法。[方法]根据GenBank公布的副猪嗜血杆菌16 S rRNA基因序列,选择其保守区域设计1对特异性引物。通过优化引物浓度和退火温度,建立快速定量检测副猪嗜血杆菌的实时荧光PCR方法,并评价了其特异性和稳定性。[结果]建立的实时荧光PCR方法最低检测限是50拷贝/μl,重复性好,变异系数均小于2%。该方法特异性强,只能检测副猪嗜血杆菌,不能检测到猪链球菌2型、金黄色葡萄球菌、大肠杆菌DH5α和猪伤寒沙门氏菌。采用该方法对10份临床疑似HPS感染样本进行检测,其结果与细菌分离培养和常规PCR的结果一致。[结论]建立的实时荧光PCR方法快速、灵敏、特异、重复性高,可用于HPS感染的临床快速检测。     

双重 PC R检测罗非鱼源无乳链球菌方法的建立

根据罗非鱼源无乳链球菌16S rRNA 基因和sip基因序列,设计、合成2对特异性引物,通过对反应体系和反应条件优化,建立快速检测无乳链球菌的双重PCR方法。该方法扩增无乳链球菌可获得1305 bp和121 bp 2个特异性片段;对6株链球菌属的菌株进行特异性分析,仅无乳链球菌能扩增出16S rRNA 基因和sip基因2条特异性条带,而海豚链球菌无条带检出;经灵敏度试验,可检测到无乳链球菌菌株070717LL的最小量为1.05＆#215;10^2 CFU ;同时,双重PCR可以检测出无乳链球菌菌株070717LL人工感染的罗非鱼脾、脑、肾组织中细菌DNA ,特别是脾脏和肾脏组织的样品检测效果好。结果证明所建立的方法具有快速、特异性强、灵敏度高等优点,适用于对罗非鱼源无乳链球菌病的流行病学调查。     

Community structure of bacteria on different types of mineral particles in a sandy soil

Various types of mineral particles in a soil probably provide different microenvironments for microorganisms. The purpose of this study is to investigate whether different types of mineral in a soil harbor different bacterial populations. DNA was extracted from five types (quartz, feldspar, pyroxene, magnetite, iron-coated reddish brown particles) of sand-size mineral particles separated from a sandy soil, and was amplified for partial 16 S rRNA gene by polymerase chain reaction (PCR). Twenty-nine to 69 amplicons per each type of mineral were cloned and sequenced, followed by phylogenetic affiliation of the sequences. As a result, some types of bacteria were detected on all of the types of mineral including the orders Rhizobiales, Bacillales, and Acidobacteriales. In the case of Acidobacteriales, higher percentages were found on magnetite and quartz. Some taxa were restricted to specific types of mineral; the class Actinobacteria was found on pyroxene but not on quartz, and rarely on magnetite and feldspar. Bacterial diversity at the order level estimated by Chao1 value was higher in feldspar and pyroxene than the other three types of mineral. The UniFrac Significance test indicated that the differences in bacterial communitiy structures among the particles were suggestive except that between feldspar and pyroxene. These results support the idea that different communities of bacteria were associated with each of the mineral types.     

条锈菌侵染早期小麦叶片RNA和rRNA的合成

 采用示踪方法研究了条锈菌侵染早期小麦叶片的RNA和rRNA合成。结果表21h期间,表现不亲和性反应的叶片总RNA合成有所增加,而亲和性反应寄主叶片则低rRNA合成未受侵染影响。在接种后39~45h期间,只有呈亲和性反应的寄主叶片RNA和大幅度增加。对rRNA各组分合成的测定表明条锈菌侵染所影响的只是大分子量rRNA,胞质和叶绿体rRNA的合成也存在差别。文中讨论了上述变化的病理学意义。     

Validation and application of real-time polymerase chain reaction assays for representative rumen bacteria

Real‐time polymerase chain reaction (PCR) assays for 11 representative rumen bacterial species were validated. The sensitivity was tested by using the serially diluted target 16S rDNA from respective bacterial species. The recovery of the target DNA and the assay reproducibility were determined using DNA from rumen fluid spiked with different quantities of the target. Minimum detection levels for the target were 10–100 copies in pure culture. The recovery of the added target ranged from 82.4 to 116.6%. The intra‐ and inter‐assay variations of each assay were <9.4 and <12.6%, respectively. Therefore, the real‐time PCR assays evaluated in the present study are considered to be sufficiently reliable for monitoring all 11 bacterial species in the rumen. The assays were then applied to the monitoring of the bacterial species attached to ruminally incubated rice straw. Among the monitored fibrolytic species, Fibrobacter succinogenes was found to be the most dominant, accounting for 2.61% of total bacteria after 24 h incubation. Selenomonas ruminantium and Streptococcus bovis, non‐fibrolytics, were detected on the rice straw at 8.96% and 1.16% of total bacteria, respectively. Such high levels of non‐fibrolytics on the plant fiber suggest a synergistic relationship between fibrolytics and non‐fibrolytics.     

Armillaria species on tea in Kenya identified using isozyme and DNA sequence comparisons

The aim of this study was to identify seven Armillaria isolates obtained from diseased tea bushes in Kenya using pectic enzyme profiles, PCR-RFLP and IGS-I DNA sequence data. The combination of these identification methods confirmed the presence of three distinct Armillaria groups. One of these groups resembled Zimbabwean group I ( A. fuscipes ). The second group was phylogenetically closely related to A. mellea ssp. nipponica . The third group was different from all other African isolates examined, but had isozyme patterns, especially of pectin methylesterases (PMEs), similar to those of isolates related to A. mellea ssp. nipponica. Analyses of sequence data suggested that this group is phylogenetically closely related to A. hinnulea from Australia and New Zealand.     

‘Candidatus Phytoplasma australiense’ is the phytoplasma associated with Australian grapevine yellows, papaya dieback and Phormium yellow leaf diseases

Sequence comparisons and phylogenetic analysis of the 16S rRNA genes and the 16S/23S spacer regions of the phytoplasmas associated with Australian grapevine yellows, papaya dieback and Phormium yellow leaf diseases revealed minimal nucleotide differences between them resulting in the formation of a monophyletic group. Therefore, along with Australian grapevine yellows, the phytoplasmas associated with Phormium yellow leaf and papaya dieback should also be considered as Candidatus Phytoplasma australiense.     

我国主要养殖罗非鱼的16S rRNA序列特征分析

对我国主要养殖的尼罗、奥利亚、莫桑比克、杂交种尼奥（尼罗♀×奥利亚♂）和红罗非鱼（莫桑比克×尼罗）的线粒体16S rRNA部分序列进行了PCR扩增和测序分析,探讨罗非鱼种间亲缘关系和种类鉴别标记。PCR产物经直接测序,5种罗非鱼中大部分个体均获得长546 bp的基因序列。其碱基组成GC含量为47.4%。序列比对分析显示变异位点18个,没有插入/缺失位点,转换/颠换比率为2.7。序列分析表明,红和奥利亚各有2个单倍型,尼奥、莫桑比克与尼罗各有1个单倍型。其中,尼奥与尼罗的单倍型序列相同,莫桑比克与红罗非鱼的1个单倍型序列相同。表明部分红罗非鱼的母本为莫桑比克。UPGMA聚类分析表明,尼奥与尼罗聚成一支、红罗非鱼与莫桑比克成一支、奥利亚独成一支。