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rpoB 是分析扩增子测序细菌群落多样性的有前途的标记。

rpoB, a promising marker for analyzing the diversity of bacterial communities by amplicon sequencing.

机构信息

DGIMI, INRA, University Montpellier, 34095, Montpellier, France.

CBGP INRA CIRAD IRD Montpellier SupAgro, Univ. Montpellier, 755 avenue du Campus Agropolis, CS 300 16, F-34988, Montferrier sur Lez cedex, France.

出版信息

BMC Microbiol. 2019 Jul 29;19(1):171. doi: 10.1186/s12866-019-1546-z.

Abstract

BACKGROUND

Microbiome composition is frequently studied by the amplification and high-throughput sequencing of specific molecular markers (metabarcoding). Various hypervariable regions of the 16S rRNA gene are classically used to estimate bacterial diversity, but other universal bacterial markers with a finer taxonomic resolution could be employed. We compared specificity and sensitivity between a portion of the rpoB gene and the V3 V4 hypervariable region of the 16S rRNA gene.

RESULTS

We first designed universal primers for rpoB suitable for use with Illumina sequencing-based technology and constructed a reference rpoB database of 45,000 sequences. The rpoB and V3 V4 markers were amplified and sequenced from (i) a mock community of 19 bacterial strains from both Gram-negative and Gram-positive lineages; (ii) bacterial assemblages associated with entomopathogenic nematodes. In metabarcoding analyses of mock communities with two analytical pipelines (FROGS and DADA2), the estimated diversity captured with the rpoB marker resembled the expected composition of these mock communities more closely than that captured with V3 V4. The rpoB marker had a higher level of taxonomic affiliation, a higher sensitivity (detection of all the species present in the mock communities), and a higher specificity (low rates of spurious OTU detection) than V3 V4. We compared the performance of the rpoB and V3 V4 markers in an animal ecosystem model, the infective juveniles of the entomopathogenic nematode Steinernema glaseri carrying the symbiotic bacteria Xenorhabdus poinarii. Both markers showed the bacterial community associated with this nematode to be of low diversity (< 50 OTUs), but only rpoB reliably detected the symbiotic bacterium X. poinarii.

CONCLUSIONS

Our results confirm that different microbiota composition data may be obtained with different markers. We found that rpoB was a highly appropriate marker for assessing the taxonomic structure of mock communities and the nematode microbiota. Further studies on other ecosystems should be considered to evaluate the universal usefulness of the rpoB marker. Our data highlight two crucial elements that should be taken into account to ensure more reliable and accurate descriptions of microbial diversity in high-throughput amplicon sequencing analyses: i) the need to include mock communities as controls; ii) the advantages of using a multigenic approach including at least one housekeeping gene (rpoB is a good candidate) and one variable region of the 16S rRNA gene. This study will be useful to the growing scientific community describing bacterial communities by metabarcoding in diverse ecosystems.

摘要

背景

微生物群落组成通常通过特定分子标记(宏条形码)的扩增和高通量测序来研究。16S rRNA 基因的各种高变区通常用于估计细菌多样性,但也可以使用具有更精细分类分辨率的其他通用细菌标记。我们比较了 rpoB 基因的一部分和 16S rRNA 基因 V3-V4 高变区的特异性和灵敏度。

结果

我们首先设计了适用于 Illumina 测序技术的 rpoB 通用引物,并构建了一个包含 45000 个序列的参考 rpoB 数据库。使用两种分析管道(FROGS 和 DADA2)从(i)革兰氏阴性和革兰氏阳性菌系的 19 株细菌的模拟群落;(ii)与昆虫病原线虫相关的细菌组合体中扩增和测序 rpoB 和 V3-V4 标记。在使用两种分析管道(FROGS 和 DADA2)对模拟群落进行宏条形码分析时,rpoB 标记所估计的多样性与这些模拟群落的预期组成更接近,而 V3-V4 标记则不然。rpoB 标记的分类归属水平更高,灵敏度(检测模拟群落中存在的所有物种)更高,特异性(假 OTU 检测率低)也更高。我们在昆虫病原线虫 Steinernema glaseri 的感染性幼虫携带共生细菌 Xenorhabdus poinarii 的动物生态系统模型中比较了 rpoB 和 V3-V4 标记的性能。两种标记都显示与这种线虫相关的细菌群落多样性较低(<50 个 OTU),但只有 rpoB 可靠地检测到共生细菌 X. poinarii。

结论

我们的结果证实,不同的标记物可能获得不同的微生物群落组成数据。我们发现 rpoB 是评估模拟群落和线虫微生物组分类结构的高度合适的标记物。应该考虑对其他生态系统进行进一步研究,以评估 rpoB 标记的普遍适用性。我们的数据突出了两个关键因素,这些因素应该考虑在内,以确保在高通量扩增子测序分析中更可靠和准确地描述微生物多样性:i)需要将模拟群落作为对照;ii)使用至少包括一个管家基因(rpoB 是一个很好的候选基因)和 16S rRNA 基因可变区的多基因方法的优势。本研究将有助于越来越多的科学社区在不同的生态系统中通过宏条形码描述细菌群落。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6fb9/6664775/ca8f9162817e/12866_2019_1546_Fig1_HTML.jpg

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