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共生藻属共生甲藻的分子定量分析。

Molecular quantification of symbiotic dinoflagellate algae of the genus Symbiodinium.

作者信息

Loram Jeannette E, Boonham Neil, O'Toole Peter, Trapido-Rosenthal Henry G, Douglas Angela E

机构信息

Department of Biology, University of York, York, YO10 5YW, UK.

出版信息

Biol Bull. 2007 Jun;212(3):259-68. doi: 10.2307/25066608.

DOI:10.2307/25066608
PMID:17565115
Abstract

The dinoflagellate microalga Symbiodinium is the dominant algal symbiont in corals and related marine animals. To explore the incidence of mixed infections, methods employing real-time quantitative polymerase chain reaction (QPCR) and fluorescence in situ hybridization (FISH) were developed. In experiments focusing on Symbiodinium clades A and B, QPCR and FISH results were well correlated and generally more precise and sensitive than those from the endpoint PCR-restriction fragment length polymorphism analysis (PCR-RFLP) traditionally used for this application, thus increasing the detected incidence of mixed infections. For example, the prevalence of mixed infections in the sea anemone Condylactis gigantea was 40% by PCR-RFLP and 80%-90% by QPCR and FISH. However, the use of QPCR and FISH was limited by inter-host variation in the rRNA gene copy number per Symbiodinium cell, precluding any single conversion factor between QPCR signal and Symbiodinium cell number; and one FISH probe that gave excellent hybridization efficiency with cultured Symbiodinium yielded variable results with Symbiodinium from symbioses. After controlling for these caveats, QPCR studies revealed that field-collected hosts previously described as universally unialgal bore up to 1.6% of the alternative clade. Further research is required to establish the contribution that algal cells at low density in symbiosis and external to the symbiosis make to the minor clade.

摘要

甲藻微藻共生藻是珊瑚及相关海洋动物中占主导地位的藻类共生体。为了探究混合感染的发生率,开发了采用实时定量聚合酶链反应(QPCR)和荧光原位杂交(FISH)的方法。在针对共生藻A和B类群的实验中,QPCR和FISH结果具有良好的相关性,并且通常比传统用于此应用的终点PCR-限制性片段长度多态性分析(PCR-RFLP)更精确、更灵敏,从而提高了混合感染的检测发生率。例如,巨型海葵中混合感染的发生率通过PCR-RFLP检测为40%,通过QPCR和FISH检测为80%-90%。然而,QPCR和FISH的使用受到每个共生藻细胞rRNA基因拷贝数在宿主间变化的限制,排除了QPCR信号与共生藻细胞数之间的任何单一转换因子;并且一种与培养的共生藻具有出色杂交效率的FISH探针,对共生关系中的共生藻产生了可变的结果。在控制了这些注意事项后,QPCR研究表明,先前被描述为普遍单一藻类的野外采集宿主中,高达1.6%含有替代类群。需要进一步研究来确定共生中低密度的藻类细胞以及共生体外的藻类细胞对次要类群的贡献。

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