【摘 要】
:
Universally conserved 16S rRNA gene sequences generated using high-throughput sequencing technique has become powerful tool to analysis the robust diversity and characterizing microbial communities.Re
【机 构】
:
Interdisciplinary Program in Bioinformatics,Seoul National University
【出 处】
:
第七届全国微生物资源学术暨国际微生物系统与分类学研讨会
论文部分内容阅读
Universally conserved 16S rRNA gene sequences generated using high-throughput sequencing technique has become powerful tool to analysis the robust diversity and characterizing microbial communities.Recently,even full-length 16S rRNA sequence can be obtained from PacBio(R)SMRT sequencer with high yield and accuracy.While partial region sequences have been used as sequence tags in microbial community analysis with sequencing bias and absence of taxonomic classification below genus level,the analysis using full-length 16S rRNA is expected to improve the result significantly.In this study,soil metagenome,fecal metagenome and a synthetic mock community DNA were profiled for bacterial 16S with SMRT sequencing using P6/C4chemistry.Triplicate 16S rDNA PCR and its representing SMRT sequencing were performed five times repeatedly.Each SMRT cell of full-length 16S rDNA reads analyzed using three different CCS filtering condition,CCS with minimum 6 full passes,minimum 90%,and 99%predicted accuracy.Bareode sorting and 12~18kbp length filtering was followed by primer trimming process.Homopolymer checked as error correction and UCHIME from USEARCH program used for detect chimeras.Non-chimeric CCS reads analyzed for community profiling through in house pipeline.CCS reads accuracy evaluated by number of mismatches and insertion/deletion errors.Mock community profile evaluated in classification rate at taxonomic levels and its accuracy,taxon composition.From soil and fecal data,we were able to sort out non-chimeric sequences based on the reproduction of highly similar sequences from multiple PCR reactions.Overall,we demonstrate the usefulness of full-length 16S rRNA gene amplicon sequencing in microbial ecology,and suggest the optimal method for generation and analysis of barcoded full-length 16S rDNA sequence data.
其他文献
The objective of this study was to investigate the endophytic microbial communities in Noni(Morinda citrifolia L.)whole plants,including the roots,branches,leaves,seeds and fruits of Noni.By using mic
Enterococcus faecalis is one of the most important species inthe genus Enterococcus.Although some isolates are considered as human pathogens,other isolates are used in food production.It is therefore
Ginsenosides are known as the main active components in ginseng and minor ginsenosides are more pharmaceutically active than major ginsenosides.Ginsenoside compound K especially exhibits anti-genotoxi
Little is known about endophytes associated with the grapevine plant inhabiting saline-alkali desertification Gobi.The diversity of endophytes was investigated from the root of Vitis vinifera collecte
Traditionally,strain types of bacteria are determined by multilocus sequence typing(MLST)of several housekeeping genes.In case of mixed population of nonculturable bacteria,generation of larg.e clone
There are a huge amount of microbial resources in desertification region of Xinjiang China,due to its special environment and less human interference.But we can only obtain the cultivated bacteria for
As a fast-growing tree species,paulownia has a wide distribution in China.Paulownia witches-broom is a main disease caused by the phytoplsama belonging to 16SrI-D subgroup in paulownia production.Aimi
Actinomycetes are outstanding collection of microorganisms with numerous affiliates reported for different kinds of bioactive features and extensive commercial importance.Several reports on the ecolog
Plant growth promoting(PGP)rhizobacteria can improve fertilizer use efficiency,reduced pathogen infection,and improved resistance to abiotic stresses such as drought,mineral deficiency and salinity.In
ACC脱氨酶(ACC deaminase)是植物促生菌中常见的一种酶,通过调节乙烯浓度和植物激素来促进植物生长帮助宿主抵抗逆境胁迫.本研究以沿海滩涂上生长的盐生植物中华补血草为植物材料,结合根际菌及植物内生菌的分离方法从中分离筛选得到23株具有ACC脱氨酶活性的菌株,对其ACC脱氨酶活性进行定量检测,有11株菌的ACC脱氨酶含量在20 μmol α-KA/(mg Pr·h)以上,其中KLBMP 5