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基于TaqMan技术对蓝藻科中含叶绿素d的蓝细菌进行快速定量分析。

Rapid TaqMan-based quantification of chlorophyll d-containing cyanobacteria in the genus Acaryochloris.

作者信息

Behrendt Lars, Nielsen Jeppe L, Sørensen Søren J, Larkum Anthony W D, Winther Jakob R, Kühl Michael

机构信息

Marine Biological Section, Department of Biology, University of Copenhagen, Helsingør, Denmark.

出版信息

Appl Environ Microbiol. 2014 May;80(10):3244-9. doi: 10.1128/AEM.00334-14. Epub 2014 Mar 14.

Abstract

Reports of the chlorophyll (Chl) d-containing cyanobacterium Acaryochloris have accumulated since its initial discovery in 1996. The majority of this evidence is based on amplification of the gene coding for the 16S rRNA, and due to the wide geographical distribution of these sequences, a global distribution of Acaryochloris species was suggested. Here, we present a rapid, reliable, and cost-effective TaqMan-based quantitative PCR (qPCR) assay that was developed for the specific detection of Acaryochloris species in complex environmental samples. The TaqMan probe showed detection limits of ~10 16S rRNA gene copy numbers based on standard curves consisting of plasmid inserts. DNA from five Acaryochloris strains, i.e., MBIC11017, CCMEE5410, HICR111A, CRS, and Awaji-1, exhibited amplification efficiencies of >94% when tested in the TaqMan assay. When used on complex natural communities, the TaqMan assay detected the presence of Acaryochloris species in four out of eight samples of crustose coralline algae (CCA), collected from temperate and tropical regions. In three out of these TaqMan-positive samples, the presence of Chl d was confirmed via high-performance liquid chromatography (HPLC), and corresponding cell estimates of Acaryochloris species amounted to 7.6 × 10(1) to 3.0 × 10(3) per mg of CCA. These numbers indicate a substantial contribution of Chl d-containing cyanobacteria to primary productivity in endolithic niches. The new TaqMan assay allows quick and easy screening of environmental samples for the presence of Acaryochloris species and is an important tool to further resolve the global distribution and significance of this unique oxyphototroph.

摘要

自1996年首次发现含叶绿素d的蓝细菌——栖热嗜温光养菌以来,相关报道不断积累。这些证据大多基于编码16S rRNA的基因扩增,由于这些序列分布广泛,因此有人认为栖热嗜温光养菌在全球范围内均有分布。在此,我们介绍一种基于TaqMan的快速、可靠且经济高效的定量PCR(qPCR)检测方法,该方法用于在复杂环境样本中特异性检测栖热嗜温光养菌。基于由质粒插入片段组成的标准曲线,TaqMan探针显示出约10个16S rRNA基因拷贝数的检测限。在TaqMan检测中对来自5株栖热嗜温光养菌菌株(即MBIC11017、CCMEE5410、HICR111A、CRS和淡路-1)的DNA进行测试时,其扩增效率>94%。当应用于复杂的自然群落时,TaqMan检测在从温带和热带地区采集的8个壳状珊瑚藻(CCA)样本中的4个样本中检测到了栖热嗜温光养菌的存在。在这些TaqMan检测呈阳性的样本中的3个样本中,通过高效液相色谱法(HPLC)确认了叶绿素d的存在,栖热嗜温光养菌的相应细胞估计数为每毫克CCA中7.6×10¹至3.0×10³个。这些数字表明含叶绿素d的蓝细菌对内生生态位的初级生产力有重大贡献。这种新的TaqMan检测方法能够快速简便地筛选环境样本中栖热嗜温光养菌的存在情况,是进一步解析这种独特的产氧光合生物的全球分布及其重要性的重要工具。

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